Mahshid Hashemkhani1, Marilena Loizidou2, Alexander J MacRobert2, Havva Yagci Acar1,3. 1. Graduate School of Materials Science and Engineering, Koç University, Rumelifeneri Yolu, Sariyer, Istanbul 34450, Turkey. 2. Division of Surgery and Interventional Science, Centre for Nanomedicine and Surgical Theranostics, University College London, Royal Free Campus, Rowland Hill Street, London NW3 2PE, U.K. 3. Department of Chemistry, Koç University, KUYTAM, Rumelifeneri Yolu, Sariyer, Istanbul 34450, Turkey.
Abstract
Silver-indium-sulfide quantum dots (AIS QDs) have potential applications in many areas, including biomedicine. Their lack of regulated heavy metals, unlike many commercialized QDs, stands out as an advantage, but the necessity for alloyed or core-shell structures and related costly and sophisticated processes for the production of stable and high quantum yield aqueous AIS QDs are the current challenges. The present study demonstrates the one-step aqueous synthesis of simple AgInS2 QD compositions utilizing for the first time either a polyethyleneimine/2-mercaptopropionic acid (AIS-PEI/2MPA) mixture or only 2-mercaptopropionic acid (AIS-2MPA) as the stabilizing molecules, providing a AgInS2 portfolio consisting of cationic and anionic AIS QDs, respectively, and tuneable emission. Small AIS QDs with long-term stability and high quantum yields (19-23%) were achieved at a molar ratio of Ag/In/S 1/10/10 in water without any dopant or a semiconductor shell. The theranostic potential of these cationic and anionic AIS QDs was also evaluated in vitro. Non-toxic doses were determined, and fluorescence imaging potential was demonstrated. More importantly, these QDs were electrostatically loaded with zwitterionic 5-aminolevulinic acid (ALA) as a prodrug to enhance the tumor availability of ALA and to improve ALA-induced porphyrin photodynamic therapy (PDT). This is the first study investigating the influence of nanoparticle charge on ALA binding, release, and therapeutic efficacy. Surface charge was found to be more critical in cellular internalization and dark toxicity rather than drug loading and release. Both QDs provided enhanced ALA release at acidic pH but protected the prodrug at physiological pH, which is critical for tumor delivery of ALA, which suffers from low bioavailability. The PDT efficacy of the ALA-loaded AIS QDs was tested in 2D monolayers and 3D constructs of HT29 and SW480 human colon adenocarcinoma cancer cell lines. The incorporation of ALA delivery by the AIS QDs, which on their own do not cause phototoxicity, elicited significant cell death due to enhanced light-induced ROS generation and apoptotic/necrotic cell death, reducing the IC50 for ALA dramatically to about 0.1 and 0.01 mM in anionic and cationic AIS QDs, respectively. Combined with simple synthetic methods, the strong intracellular photoluminescence of AIS QDs, good biocompatibility of especially the anionic AIS QDs, and the ability to act as drug carriers for effective PDT signify that the AIS QDs, in particular AIS-2MPA, are highly promising theranostic QDs.
Silver-indium-sulfide quantum dots (AIS QDs) have potential applications in many areas, including biomedicine. Their lack of regulated heavy metals, unlike many commercialized QDs, stands out as an advantage, but the necessity for alloyed or core-shell structures and related costly and sophisticated processes for the production of stable and high quantum yield aqueous AIS QDs are the current challenges. The present study demonstrates the one-step aqueous synthesis of simple AgInS2 QD compositions utilizing for the first time either a polyethyleneimine/2-mercaptopropionic acid (AIS-PEI/2MPA) mixture or only 2-mercaptopropionic acid (AIS-2MPA) as the stabilizing molecules, providing a AgInS2 portfolio consisting of cationic and anionic AIS QDs, respectively, and tuneable emission. Small AIS QDs with long-term stability and high quantum yields (19-23%) were achieved at a molar ratio of Ag/In/S 1/10/10 in water without any dopant or a semiconductor shell. The theranostic potential of these cationic and anionic AIS QDs was also evaluated in vitro. Non-toxic doses were determined, and fluorescence imaging potential was demonstrated. More importantly, these QDs were electrostatically loaded with zwitterionic 5-aminolevulinic acid (ALA) as a prodrug to enhance the tumor availability of ALA and to improve ALA-induced porphyrin photodynamic therapy (PDT). This is the first study investigating the influence of nanoparticle charge on ALA binding, release, and therapeutic efficacy. Surface charge was found to be more critical in cellular internalization and dark toxicity rather than drug loading and release. Both QDs provided enhanced ALA release at acidic pH but protected the prodrug at physiological pH, which is critical for tumor delivery of ALA, which suffers from low bioavailability. The PDT efficacy of the ALA-loaded AIS QDs was tested in 2D monolayers and 3D constructs of HT29 and SW480 human colon adenocarcinoma cancer cell lines. The incorporation of ALA delivery by the AIS QDs, which on their own do not cause phototoxicity, elicited significant cell death due to enhanced light-induced ROS generation and apoptotic/necrotic cell death, reducing the IC50 for ALA dramatically to about 0.1 and 0.01 mM in anionic and cationic AIS QDs, respectively. Combined with simple synthetic methods, the strong intracellular photoluminescence of AIS QDs, good biocompatibility of especially the anionic AIS QDs, and the ability to act as drug carriers for effective PDT signify that the AIS QDs, in particular AIS-2MPA, are highly promising theranostic QDs.
Semiconductor quantum
dots (QDs) have attracted great interest
as a novel class of promising optical probes in the past two decades.[1,2] Compared to bulk materials, they exhibit many advantages, such as
size-dependent photoluminescence (PL), high PL quantum yields (QY),
sharp and symmetrical fluorescence peaks, broad excitation spectra,
large Stokes shifts, and long-lasting luminesce, which is valuable
for medical imaging.[3,4] Recently, heavy metal-free ternary
I–III–VI2 QDs such as CuInS2,[5] CuInSe2,[6] and AgInS2[7,8] have been intensively investigated.
AgInS2 (AIS) QDs are promising due to their relatively
wide bandgaps ranging from 1.87 to 2.03 eV that provide tunable luminescence
in the visible region, especially in the optical window from 600 to
800 nm suitable for medical imaging.[6,8,9] Besides, a more stable nature and synthesis at lower
temperatures are important advantages of AIS over CuInS2, making it attractive for medical purposes. However, the synthetic
procedures for high-quality ternary I–III–VI2 QDs usually involve non-polar organic solvents, which might limit
the direct applications of these QDs in biological applications.[8−11] Often, quaternary compositions with Zn or core–shell structures
(AIS/ZnS) are preferred to improve the QY and stability.[12−15] However, this strategy usually causes a blue shift in the emission
wavelength due to the wider bandgap of ZnS, which may not always be
suitable for applications, e.g., for optical imaging best achieved
between 600 and 900 nm. Moreover, the complexity and cost of these
organic routes and hydrophobicity of the produced QDs are significant
issues in large production and for application in biotechnology and
medicine wherein aqueous colloidal particles are needed.The
transfer of the hydrophobic QDs into the aqueous phase is usually
achieved by post-synthetic ligand exchange or by phase-transfer using
amphiphilic copolymers, which causes a significant drop in QY.[10,11,16] Alternative aqueous synthetic
protocols usually cause low QY, hence almost always, a ZnS shell or
Zn–Ag–In–S (ZAIS) quaternary systems are preferred.[7,10,17,18] Deng et al.[7,17] produced glutathione (GSH)-coated
ZAIS QDs in water with tunable PL in the range of 550–605 nm
and QY between 10 and 30% (with respect to R6G). Luo et al.[19] synthesized GSH-coated AIS nanocrystals in water
at 95 °C with a maximum QY of 3%. They investigated the influence
of pH, GSH/In, In/Ag, and In/S ratios on the optical properties of
AIS. It was shown that pH 8.5 and a high GSH/In ratio could increase
the PL intensity (peak position was not changed), whereas the ratios
of In/Ag and In/S could affect the emission wavelength and intensity.
Recently, we managed to produce stable GSH-coated AIS QDs without
Zn, emitting at 634 nm with a 21% QY by applying a cation-rich formulation
and avoiding large excess use of GSH (Ag/In/S/GSH 1/4/2.5/10 mole
ratio).[3]Xu et al. applied hydrothermal
synthesis to produce cysteine-coated
AIS/ZnS with QY of as high as 35% using thioacetamide (TAA) to control
the growth rather than the fast sulfur-releasing Na2S.[20] Recently, Mrad et al. reported 3-mercaptopropionic
acid (3MPA)-coated AIS QDs with 5.5–15.6% QY and AIS/ZnS with
up to 78% QY after fractionation of the products.[8] The key roles of 3MPA were reported as sulfur release at
high temperatures, ability to form a ligand–cation complex
with both In3+ and Ag+, and bidentate binding
to the surface, causing passivation of the chalcogenide vacancies.
One additional important point would be the lack of emission tunability
of AIS unless zinc was added. Regulacio et al. applied polyacrylic
acid (PAA) and mercaptoacetic acid (MAA) simultaneously to improve
the QY of the aqueous AIS/ZnS QDs to 20%.[21] However, the use of only MAA or PAA provided very poor luminescence.
They suggested that polyacrylic acid would bind In3+ and
regulate its reactivity, whereas the thiol of MAA would bind Ag+. Another critical function of PAA was also reported as enhancing
the colloidal stability of these QDs because the aqueous AIS QDs also
lack long-term stability.[19,22,23] Indeed, utilization of the PAA/MAA-mixed coating approach was first
reported by our group to improve the colloidal stability of the MAA-coated
CdS while maintaining strong luminescence.[24]To the best of our knowledge, there are only two examples
of cationic
aqueous AIS QDs. Raevskaya et al.[25] reported
the preparation of branched polyethyleneimine (PEI-25 kDa)-coated
AIS QDs with emission maxima at 590 nm and maximum QY of 20% (with
respect to anthracene) when a Ag/In/S ratio of 1/5/5 was used but
only after 2 h post-synthesis thermal treatment at 100 °C. They
have also reported the formation of about 100 nm aggregates. Wang
et al.[26] used high amounts of lower molecular
weight PEI (10 kDa) and a pressure cooker (120 °C) to produce
cationic AIS QDs (10 kDa) with yellow luminescence (emission maxima
at 560 nm) and 32% QY in small hydrodynamic sizes (18.1 nm) using
a Ag/In/S mole ratio of 1/16/10. They could not achieve emission wavelength
tuning by changing any of the variables. They attributed this to the
lack of sulfur-containing ligands, hence many S-vacancies. Therefore,
there is still a clear need to develop simple, economical, aqueous
synthetic protocols for the preparation of functional, stable, and
highly luminescent AIS with emission at and above 600 nm for medical
applications. To achieve this, the coating molecules should be selected
carefully, and the stoichiometry of the components should be optimized.
Here, we do propose 2-mercaptopropionic acid (2MPA) to produce an
anionic and PEI (25 kDa)/2MPA mixture to produce cationic AIS QDs
with long-term stability, tunability, and strong luminescence. We
have previously demonstrated the advantage of using the PEI/2MPA mixture
over the PEI coating on the luminescence properties of Ag2S QDs and on improving the biocompatibility of the cationic particles.
Polymeric coating molecules provide colloidal stability due to multidentate
binding to the nanocrystal surface but produce poor luminescence due
to the lack of effective surface passivation and surface defects.[24,27,28] However, if they are mixed with
small, thiolated molecules that can reach the surface, bind strongly,
and reduce defects, both good stability and strong luminescence may
be achieved.[24,28] Likewise, the advantage of 2MPA
over 3MPA in enhancing the luminescence intensity and colloidal stability
due to the stability of 2MPA and energetically favorable bidentate
surface binding compared to 3MPA has been demonstrated on CdS QDs,
and this approach was successfully utilized in Ag2S QDs
by our group, as well.[29] We suggest that
these coating molecules and the stabilization strategy could also
provide small, stable, strongly luminescent AIS QDs without the Zn
dopant or ZnS shell and produce an AIS portfolio with opposite surface
charges and emission in the medical imaging window.Achievement
of such aqueous cationic and anionic AIS QDs with the
emission in the visible region that can be prepared with either 2MPA
or 2MPA/PEI in surface charge would facilitate their evaluation in
nanomedicine. Currently, evaluation of AIS or ZAIS QDs in medicine
is quite limited and mostly focuses on toxicity evaluation and in
vitro.[10,11,21] Here, these
AIS QDs are also evaluated as a theranostic agent for photodynamic
therapy (PDT).PDT is a light-based medical treatment that relies
on the retention
of photosensitizers (PSs) in tumor tissues, which can be activated
at a specific wavelength to provide a therapeutic effect at the irradiated
area. PSs activated by a specific wavelength in the presence of molecular
oxygen generate singlet oxygen and other reactive oxygen species (ROS),
which are cytotoxic to the nearby cells due to the rapid and dramatic
increase in oxidative stress.[30−32] Hence, PDT is quite effective
in eliminating various pathogens such as viruses and bacteria as well
as cancer cells and therefore has found use in a variety of areas
including dermatology, ophthalmology dentistry, cosmetics, treatment
of some cancers, microbial/viral infections/biofilms, and sterilization.
In addition, photochemical internalization (PCI) of toxic drugs has
become an attractive strategy.[33−39]5-Aminolevulinic acid (ALA) is a prodrug and the precursor
of protoporphyrin
IX (PpIX), a natural PS and an intermediate in the heme biosynthesis
pathway.[40−42] ALA is clinically approved for PDT and fluorescence-based
photodiagnosis of different cancers due to the efficient metabolism
of the fluorescent PpIX photosensitizer in the malignant tumor cells.
In clinical practice, red wavelengths are typically employed for ALA-PDT,
whereas fluorescence photodiagnostic imaging typically uses blue light
excitation. However, ALA has relatively low bioavailability and cellular
uptake owing to its zwitterionic nature. Hence, its derivatization
and loading to nanoparticles have been proposed for better therapeutic
outcomes. Preparation of ALA derivatives with improved bioavailability
and lipophilicity via esterification, their peptide esters, and dendritic
and liposomal formulations have been investigated.[43−45] Chung et al.
increased the cellular uptake of ALA by conjugating it to methoxy
polyethylene glycol/chitosan.[46] Indeed,
the utilization of nanoparticles in ALA-based PDT improves the stability
of PS and could also be tuned to deliver it to the target cells in
high concentration to improve the therapeutic effect and evade the
efflux transporters that mediate drug resistance.[47] Wang et al.[48] increased the
circulation time and stability of ALA by loading it into HER2-targeted
aldehyde-functionalized hyaluronic acid and hydroxyethyl chitosan
nanoparticles. They showed that less than 40% of ALA was released
at physiological pH after 45 h, whereas the half-life of free ALA
under the same conditions is less than an hour.[48]ALA may be conjugated to the nanoparticles, or it
may be electrostatically
loaded to the charged nanoparticles.[46,49] One advantage
of electrostatic loading is the fact that it can be done in fewer
steps. Procedures involving multiple solvent exchanges, surface functionalization,
washing, etc., usually negatively affect the luminescence intensity
and hydrodynamic size of QDs. Another advantage of electrostatic loading
is pH-dependent, quick release with higher efficiency, especially
in acidic media, which is important for clinical applications. The
few examples of electrostatic loading in the literature utilized the
positively charged gold nanoparticles.[49,50]We suggest
that ALA can be loaded electrostatically to both the
cationic and anionic nanoparticles due to its zwitterionic nature.
Yet, there are no studies comparing the cationic versus anionic nanoparticles
as the delivery vehicles for ALA. The charge of the nanoparticle would
impact the biodistribution, dark toxicity, and probably the binding
and release efficiency of ALA, which are critical in ALA delivery
with nanoparticles for improved PDT efficacy. The current studies
related to the relationship between the cellular uptake and physicochemical
properties of the nanoparticles in the absence of targeting agents
imply that the access of QDs into the cells is principally governed
by the size and charge of the nanoparticles.[51,52] The negatively charged proteoglycans are supposed to attract the
positively charged QDs toward the cell membrane, causing an increased
endocytic uptake of the cationic nanoparticles but repelling the negatively
charged ones resulting in a lower uptake.[53] However, this is still disputed because some papers report that
the negatively charged nanoparticles are endocytosed more than the
positively charged QDs, whereas other studies show no correlation
of the QD surface charge.[54−56] In the present study, using AIS
with different coatings provides a great tool to answer these questions.Herein, we developed both the cationic and anionic AIS QDs with
strong luminescence in one-step aqueous synthesis without Zn incorporation
or ZnO shell, simply by utilizing either PEI/2MPA or 2MPA as the stabilizers
and loading them with ALA as the potential theranostic agents for
tumor therapy. With this design, the QDs will, in principle, protect
the ALA and enable its accumulation in the tumors due to the EPR effect
and endocytic cell internalization and provide a strong and long-lived
QD-based luminescence highlighting the region of accumulation and
favor the ALA release in the tumors selectively, hence causing a significant
increase in the tumor PpIX levels, which will lead to enhanced cell
death when irradiated.[28]The AIS
QDs prepared from silver nitrate, indium(III) nitrate,
and sodium sulfide in different Ag/In/S/coating ratios provide the
stable cationic and anionic AIS QDs emitting from green to orange-red.
Bandgap and Urbach energies were determined to correlate the size,
size distribution, defects, and emission wavelength of the particles.
Long-term emission stability, as well as the colloidal stability,
was monitored. Then, in vitro fluorescence, cytotoxicity, and cell
internalization of the cationic and anionic AIS QDs were examined
in the 2D and 3D-spheroid models of the HT29, HeLa, SW480, and HCT116
cancer cell lines. Finally, the potential for ALA-based PDT was investigated,
and the cationic and anionic AIS QDs as the delivery vehicles of ALA
were compared. The ALA loading and pH-dependent release efficiency
from both the QDs and PDT efficiency of the AIS/ALA QD compositions
upon 5 min 420 nm (UV lamp) irradiation were examined (Scheme a).
Scheme 1
(a) Use of the ALA-Loaded
Cationic and Anionic AIS QDs for Visible
Light PDT Coupled with QD-Based Optical Imaging in the Medical Imaging
Window. Synthesis of (b) AIS-2MPA and (c) AIS-PEI/2MPA QDs
Overall, the results demonstrate that the 2MPA
and PEI/2MPA coatings
do successfully stabilize the AIS QDs to provide small, stable QDs
with strong emission; such QDs have strong luminescence in the optical
imaging window, and ALA may be effectively loaded and released from
both, and the QD-delivered ALA provides greater phototoxicity to the
cancer cell lines. The promising results have opened possibilities
for the bio-labeling and image-guided PDT of cancer utilizing these
AIS/ALA QDs, which may be adopted to deliver other therapeutic cargos.
Experimental Section
Materials
Silver
nitrate (AgNO3), In(NO3)3·xH2O, and branched
polyethyleneimine (PEI) (Mw 25 kDa) were purchased from Sigma-Aldrich
(Germany). Sodium sulfide (Na2S) was purchased from Alfa-Aesar.
Sodium hydroxide (NaOH), 2-mercaptopropionic acid (2MPA), ethanol,
and acetic acid (CH3COOH) were purchased from Merck (USA).
5-Aminolevulinic acid hydrochloride (ALA) was bought from Research
Products International (RPI-USA). The LDS 798 near-IR laser dye was
purchased from Exciton, Inc., (USA). Ultracentrifuge tubes with polysulfone
filtration membranes (3 kDa) were purchased from Sartorius (Germany).
All chemicals were of analytical grade and used without any further
purification.The Roswell Park Memorial Institute (RPMI) 1640
and McCoy’s 5A (modified) medium were obtained from Multicell,
Wisent Inc. (Canada). The 10× minimum essential medium (MEM)
(used as the color/pH indicator) and HEPES buffer solution were purchased
from Gibco by Life Technologies, Thermo Fisher Scientific (UK). Fetal
bovine serum and l-glutamine were purchased from Capricorn
Scientific GmbH (Germany). 80% Rat Tail Collagen Type I was bought
from First Link UK Ltd. Trypsin–EDTA and penicillin–streptomycin
solutions were bought from Wisent Inc. (Canada). Thiazolyl blue tetrazolium
bromide (MTT), Alamar blue, and phosphate buffered saline (PBS) tablets
were purchased from Biomatik Corp. (Canada). Paraformaldehyde solution
4% in PBS was obtained from Santa Cruz Biotechnology, Inc. (USA).
96-well plates were purchased from Nest Biotechnology Co. Ltd. (China).
The human epithelial carcinoma cell line (HeLa), HT29, and SW480 cells
were provided by Gozuacik Lab (Sabanci University, Istanbul, Turkey)
for this study. HCT116 cells were purchased from ATCC (Ireland).
Synthesis of AIS-2MPA QDs
The 2MPA-coated AIS QDs were
prepared at different Ag/In and Ag/S ratios as summarized in Table , keeping the 2MPA/cation
mole ratio fixed at 5. All the reactions were performed under argon
and at room temperature (RT). Briefly, 2MPA in the desired amounts
based on the stoichiometries listed in Table (2MPA/S: 1/0.25–1/3.3 molar ratio)
was dissolved in 75 mL deoxygenated water in a round bottom flask.
The pH of this solution was adjusted to 7.5 using NaOH and CH3COOH solutions (1 M), and then AgNO3 and In(NO3)3·xH2O were added.
As an example, 0.022 mmol AgNO3, 0.22 mmol In(NO3)3·xH2O, and 1.2 mmol
2MPA were utilized for a molar ratio of Ag/In 1/10. The pH of the
final solution was adjusted to 7.5 and then charged with a 25 mL aqueous
solution of Na2S (0.22 mmol Na2S for a molar
ratio of Ag/In/S 1/10/10) under vigorous mechanical stirring at 500
rpm. The samples were removed from the reaction mixture at different
time points to track the particle growth. The prepared quantum dot
solutions were washed with deionized water using the centrifugal filters
(3 kDa cut off) and stored in the dark at 4 °C (Scheme b).
Table 1
Effects
of the Different Reaction
Variables on the Properties of the AIS-2MPA QDs
sample
AIS-2MPA-1
AIS-2MPA-2
AIS-2MPA-3
AIS-2MPA-4
AIS-2MPA-5
Ag/S ratio
1/10
1/2.5
1/10
1/1.25
1/10
Ag/In ratio
1/4
1/4
1/10
1/4
1/2
cation/S ratio
0.5
2
1.1
4
0.3
λemia (nm)
634
660
630
701
649
bandgap (eV)
2.10
2.13
2.15
2.34
2.15
Eub (meV)
172
168
170
137
161
FWHMc (nm)
161
190
80
203
219
Dh-numberd (nm)
46.1 ± 1.6
5.2 ± 1.1
103.7 ± 2.4
22.6 ± 2.5
Dh-intensitye (nm)
80.7 ± 10.3
38.2 ± 11.2
117.9 ± 20.1
67.9 ± 5.7
zeta potential (mv)
–38.1 ± 5.2
–42.1 ± 1.9
–43.8 ± 3.1
–41.6 ± 4.4
QY (%)
10.6 ± 2.1
19.4 ± 2.7
5.6 ± 2.1
4.9 ± 0.9
Emission maxima.
Urbach energy.
Full-width at half-maximum of the
emission peak.
Hydrodynamic
diameter measured by
DLS and reported as the number average.
Hydrodynamic diameter measured by
DLS and reported as the intensity average.
Emission maxima.Urbach energy.Full-width at half-maximum of the
emission peak.Hydrodynamic
diameter measured by
DLS and reported as the number average.Hydrodynamic diameter measured by
DLS and reported as the intensity average.
Synthesis of AIS-PEI/2MPA QDs
The PEI/2MPA-coated AIS
QDs were prepared at different Ag/In and Ag/S ratios as summarized
in Table at a coating/cation
mole ratio of 5. All the reactions were performed under argon and
at RT. The 4/1 mole ratio of PEI/2MPA was used in all the reactions
based on the amine/thiol content of the species. The cation sources
(AgNO3, In(NO3)3·xH2O) and Na2S were dissolved in 75 and 25 mL
of deoxygenated water, respectively, in separate round bottom flasks.
In a typical reaction for a molar ratio of Ag/In/S 1/10/10, 0.2 mmol
PEI and 0.05 mmol 2MPA were added to the 0.022 mmol AgNO3 and 0.22 mmol In(NO3)3·xH2O solution. The pH of the final solution was adjusted
to 9 using NaOH and CH3COOH solutions (1 M). Na2S solution (0.22 mmol Na2S for a molar ratio of Ag/In/S
1/10/10) was added to this reaction mixture under vigorous mechanical
stirring at 500 rpm. The samples were removed during the reaction
at different time points to follow the particle growth. In the end,
the quantum dot solutions were washed and kept as described above
(Scheme c).
Table 2
Effect of the Different Reaction Variables
on the Properties of the AIS-PEI/2MPA QDs
sample
AIS-PEI/2MPA-1
AIS-PEI/2MPA-2
AIS-PEI/2MPA-3
AIS-PEI/2MPA-4
AIS-PEI/2MPA-5
AIS-PEI/2MPA-6
AIS-PEI/2MPA-7
Ag/S ratio
1/10
1/10
1/2.5
1/10
1/5.5
1/1.25
1/10
Ag/In ratio
1/10
1/4
1/4
1/0.25
1/10
1/4
1/2
cations/S
ratio
1.1
0.5
2
0.5
2
4
0.3
λemia (nm)
617
640
618
774
618
655
638
bandgap
(eV)
2.74
2.4
2.57
2.02
2.15
2.12
2.24
Eub (meV)
138
149
144
167
168
151
150
FWHMc (nm)
147
177
147
105
139
240
189
Dh-numberd (nm)
7.7 ± 0.9
12.7 ± 0.4
10.5 ± 0.6
11.9 ± 0.4
8.2 ± 1.3
57.9 ± 3.7
Dh-intensitye (nm)
27.9 ± 4.1
26.3 ± 2.2
37.9 ± 10.3
60.4 ± 6.8
17.6 ± 8.7
99.1 ± 10.3
zeta potential (mV)
10.7 ± 2.1
8.1 ± 1
9.8 ± 0.3
16.4 ± 0.9
20.9 ± 3.2
–4.9 ± 1.7
QY (%)
20.3 ± 1.4
15.6 ± 0.9
7.9 ± 0.4
Emission maxima.
Urbach energy.
Full-width at half-maximum of the
emission peak.
Hydrodynamic
diameter measured by
DLS and reported as the number average.
Hydrodynamic diameter measured by
DLS and reported as the intensity average.
Emission maxima.Urbach energy.Full-width at half-maximum of the
emission peak.Hydrodynamic
diameter measured by
DLS and reported as the number average.Hydrodynamic diameter measured by
DLS and reported as the intensity average.
Characterization
X-ray photoelectron spectroscopy (XPS)
using Thermo Scientific K-Alpha XPS with Al K-alpha monochromatic
radiation (1486.3 eV) was used for compositional analysis of the crystals.
The dried samples were placed on an adhesive carbon tape and exposed
to 400 μm X-ray spot size with 50.0 eV pass energy, corresponding
to a resolution of roughly 0.5 eV. All the spectra were corrected
with respect to the C1s peak at 284.5 eV. To determine the crystal
structure of the AIS QDs, a Bruker D2 Phaser Benchtop X-ray Diffraction
(XRD) system with Cu K-α radiation (λ = 1.5406 Å)
was used between 2θ angles of 10 and 80°. The hydrodynamic
sizes, zeta potentials, and polydispersity index (PDI) of the colloidal
AIS QDs were assessed with a Malvern zetasizer nano ZS. The Ag and
In contents of the colloidal AIS QDs were determined quantitatively
by Agilent 7700x Inductively Coupled Plasma Mass Spectrometry (ICP-MS)
after the samples were treated with nitric acid:sulfuric acid (9:1
v/v). This was performed after sterile filtration of the colloidal
solutions to have the exact concentrations used in the in vitro studies.
The functional group analysis of the QDs was performed on a Thermo
Scientific Nicolet iS10 instrument (FTIR) in the wavenumber region
from 650 to 4000 cm–1 with resolution 4 cm–1. The organic content of the QDs was measured by thermogravimetric
analysis (TGA, TGA 500). The samples were heated from RT to 1000 °C
at a heating rate of 10 °C/min under a nitrogen atmosphere.The photoluminescence (PL) spectra of the AIS QDs in the range of
500–900 nm were recorded on an Agilent Cary Eclipse Fluorescence
Spectrophotometer at 480 nm excitation. The PL lifetimes were measured
using an Edinburgh FLS100 Spectrometer. The absorbance spectra were
recorded using a Shimadzu UV-3600 spectrophotometer in the 300–1000
nm range. The QY was calculated based on the procedures in the literature
using Rhodamine 6G as reference according to the following equation:[24]Grad is the ratio of the
fluorescence intensity to the absorbance of the corresponding sample,
and n is the refractive index of the solvent.
Cell Culture
All culture media were supplemented with
10% fetal bovine serum, 2% l-glutamine (200 mM), and 1% penicillin–streptomycin.
HT29, SW480, and HCT116 were cultured in McCoy’s, and HeLa
cells were cultured in the RPMI 1640 complete medium in a 5% CO2-humidified incubator at 37 °C.
Formation of 3D Spheroid
Constructs
The in vitro 3D-spheroid
constructs were prepared following the protocol from RAFT 3D culture
systems (Lonza, Slough, UK). The hydrogels were prepared from a mixture
containing 10% 10× MEM (used as the color/pH indicator) and 80%
Rat Tail Collagen Type I (First Link UK Ltd. Custom Bio-Reagents)
and neutralized with a solution made from 1.65 M NaOH and 840 mM HEPES
buffer (Thermo Fisher Scientific). The cells were seeded into the
collagen at densities of 50,000 cells for the spheroid constructs
at overall (cells and collagen mix) volumes of 240 μL per well
in a 96-well plate. The constructs were incubated at 37 °C for
15 min to set before being subjected to plastic compression using
absorbers (Lonza) for a further 15 min at RT. After the removal of
the absorbers, fresh medium was added, and the wells were placed into
the incubator.
Cytotoxicity Assay
The MTT metabolic
activity assay
was used to determine the dark cytotoxicity of the AIS-2MPA and AIS-PEI/2MPA
QDs. All the QD colloidal solutions were sterilized by passing through
sterile 0.2 μm filters. HT29, HeLa, SW480, and HCT116 cells
were seeded into a 96-well plate at a density of 12,500 cells/well
and cultured at 37 °C in a 5% CO2 atmosphere. The
medium was replaced with a fresh medium after an overnight exposure
with the QDs in cation concentrations of 0.025–100 μg/mL
as determined by ICP analysis. After 48 h incubation, the medium was
replenished, and the cells were washed with 3× PBS. After the
addition of 50 μL of MTT reagent (5 mg/mL) and 150 μL
medium to each well, purple formazan crystals formed in 4 h. The cells
were washed with 3× PBS, and then the crystals in each well were
dissolved with ethanol:DMSO (1:1 v/v) solution by shaking gently for
15 min. Relative cell viability was determined based on the absorbance
intensity measured at 600 nm with a reference reading at 630 nm using
a microplate reader (BioTek ELx800 Absorbance Microplate Reader).
Cells with no treatment were used as controls. Treated cells without
the MTT reagent were used for the correction of the absorbance intensities.
Cell Uptake and Imaging
The first experiments were
performed on the 2D cell culture and then on the 3D spheroids consisting
of multicellular aggregates that grew over 7 days before treatment.
HT29, HeLa, SW480, and HCT116 cells were seeded on 3 mL glass-bottom
petri dishes at a density of 1.75 × 105 cells/well
in a complete medium and grown for 24 h at 37 °C and 5% CO2. On the next day, the growing cells were incubated with nanoparticles
at 50 and 2 μg/mL cation concentrations of AIS-2MPA-3 and AIS-PEI/2MPA-1
QDs for 24 h. Then, the medium was replenished, and the cells were
washed with 3× PBS and were fixed with paraformaldehyde solution
(4% in PBS) for 20 min. After being washed with PBS, the cells were
incubated for an additional 15 min with 2 μg/mL of DAPI nucleus
dye. The cells were rewashed three times with PBS to remove the unbound
dye and left in 2 mL PBS to prevent drying. Cells without any QD treatment
were used as controls. The fixed cell samples were examined using
a confocal microscope (Leica dmi8/SP8) with different filters for
Alexa 488 (λexc: 488 nm and λem:
580–780) and DAPI (λexc: 325–375 nm
and λem: 435–485 nm). The same experimental
procedure was also performed for the control cells that were not treated
with the nanoparticles. Images were processed and merged using the
ImageJ analysis program.The quantitative analysis of QD uptake
was performed by the determination of cation (Ag and In) content in
the QD-treated cells. HT29, HeLa, SW480, and HCT116 cells were prepared
similarly as for microscopy image analysis and incubated with the
QD samples for 24 h. Then, the cells were washed with PBS to remove
the un-internalized nanoparticles, and after trypsinization, the supernatant
was collected. An acid digestion procedure (suprapur nitric acid 65%
and suprapur sulfuric acid 96%) was performed, and the cation concentration
of each sample was determined by ICP-MS (n = 3).To determine the intracellular localization of the QDs within the
3D constructs, separate constructs of HT29 and SW480 cell lines were
prepared (50,000 cells/model). The constructs were incubated with
AIS-2MPA-3 (50 and 2 μg/mL [cations]) and AIS-PEI/2MPA-1 (2
μg/mL [cations]) and their ALA conjugates for 24 h. The constructs
were washed with PBS three times and incubated with PBS for fluorescence
imaging using an Olympus fluorescence microscope (10× objective,
Olympus BX63) with the following filters: BF (λexc: 345 nm and λem: 455) and TRITC (λexc: 545 nm and λem: 620 nm). Samples without QD treatment
served as a control.
Electrostatic Loading of ALA to AIS QDs
ALA at a concentration
of 3 mg/mL was dissolved in 20 mM HEPES buffer, and its pH was adjusted
to 7.2–7.4 and finally filtered from a 0.2 μm filter.
The AIS-2MPA-3 and AIS-PEI/2MPA-1 QDs were also, separately, filtered
from a 0.2 μm filter. Subsequently, the 0.3 and 0.5 mmol ALA
solutions were mixed with 1 mmol AIS-2MPA-3 and AIS-PEI/2MPA-1 suspensions
and stirred at RT for 15 min. ALA amounts were calculated as 30 and
50 mol % of the functional groups available on the QDs, which was
determined by TGA. After loading, the nanoparticles were stored at
4 °C.
Isothermal Titration Calorimetry (ITC)
An isothermal
titration calorimeter (Affinity ITC, USA) was used to measure the
enthalpy changes resulting from the interaction between ALA and either
AIS-2MPA or AIS-PEI/2MPA QDs. One milliliter aliquots of either QD
or ALA solution (1 mg/mL, pH 7.4) were injected sequentially into
a 1.5 mL titration cell every 10 s. The temperature of the solution
in the titration cell was maintained at 25 °C throughout the
experiments. The results are reported as the change in enthalpy per
titration (μcal) versus the concentration of the added ALA after
each injection.
ALA Release Profile
The release
of the loaded ALA from
the AIS QDs was investigated at pH 5.5 and 7.4 at 37 °C. Typically,
5 mL AIS-2MPA-3-50%ALA or AIS-PEI/2MPA-1-50%ALA was added to a dialysis
bag (MWCO 3500) and immersed in 500 mL of PBS (pH 5.5 or 7.4) with
constant shaking (100 rpm) at 37 °C. At fixed time intervals,
3 mL of the released solution was removed, and 3 mL fresh PBS medium
was added. The amount of ALA in the removed samples was determined
by absorbance at 263 nm and using a concentration-dependent absorbance
standard curve prepared for ALA in PBS (pH 5 or 7.4).
Measurement
of PpIX Formation
HT29, HeLa, SW480, and
HCT116 cells were seeded at a density of 12,500 cells/well in the
96-well plates and incubated for 24 h in a complete medium. The medium
of some wells containing the cells was then replaced with a serum-free
medium containing 0.002–0.688 mM ALA to be used as control,
whereas the other wells were subjected to AIS-2MPA-3 and AIS-PEI/2MPA-1
containing the corresponding amount of ALA. Untreated cells were used
as the drug-free control. The fluorescence intensity was measured
using a Synergy H1 microplate reader (Biotek) at an excitation and
an emission wavelength of 420 and 635 nm, respectively, after 24 h
incubation with ALA or nanoparticles.
PDT Studies
For
the in vitro PDT studies, HT29 and
SW480 cells were seeded at a density of 12,500 cells/well (2D cell
culture) and 50,000 cells/well (3D models) in 96-well plates and cultured
as described above for 24 h (the 2D cell cultures) and 7 days (3D
models). The QDs containing different concentrations of ALA in the
range of 0.018–0.688 mM were added to each well and incubated
for 24 h. Then, the medium was substituted with a serum-free medium,
and each well was illuminated with a blue LumiSource-flatbed lamp
with a peak emission at 420 nm and 7 mW/cm2 output (PCI
Biotech, Oslo, Norway) from the bottom of the plate for 5 min. The
light-irradiated cells were then incubated for another 24 h before
cell viability was determined using the standard MTT protocol for
the 2D cell cultures and the fluorescence-based Alamar blue assay
for the 3D models, which is the appropriate assay to use for light
scattering constructs. The viability of cells that were treated the
same way except laser treatment was also determined. Cells that were
not treated with no ALA or QD treatment were used as controls.
Intracellular
ROS Generation
To assess ROS generation
as a result of irradiation, HT29 and SW480 cells were seeded in the
96-well plate at a density of 12,500 cells/well (2D cell cultures)
and incubated in complete media for 24 h. Then, QDs were added to
the cells at cation concentrations of 50 and 2 μg/mL of AIS-2MPA-3
and AIS-PEI/2MPA-1 QDs for 24 h, respectively. The cells were then
also irradiated using a blue LumiSource-flatbed lamp with peak emission
at 420 nm and 7 mW/cm2 output (PCI Biotech, Oslo, Norway)
for 5 min and incubated for another 24 h. The ROS levels of the treated
cells were determined using the Enzo Total ROS Detection Kit following
the manufacturer’s instructions using a Synergy H1 microplate
reader (Biotek) at an excitation/emission wavelength of 485/538 nm.
Live/Dead Assay
A live/dead cell viability assay (Thermo
Fisher Scientific, UK) was utilized to determine the live and dead
cell population after the ALA, QD, and ALA-loaded QD treatment before
and after irradiation. HT29 and SW480 cells were seeded following
the procedure explained for the ROS assay. After irradiation at 420
nm for 5 min, the cells were stained with the live/dead assay based
on the protocol that is provided by the manufacturer. Finally, images
were collected using an inverted fluorescence microscope (EVOS FL
color, Life Technologies, Thermo Fisher Scientific, UK).
Termination
of Apoptosis/Necrosis
The Annexin V-FITC
apoptosis detection kit (Abcam, UK) was used to confirm the mechanism
of cell death in the 2D and 3D models. The cells were seeded as described
above. At 24 h after being exposed to irradiation at 420 nm, 100 μL
of 1× binding buffer was added to the models in each well before
adding 1 μL of Annexin V-FITC (Ex/Em 488/525 nm) and 5 μL
of propidium iodide (Ex/Em 535/617 nm) to the buffer solution in each
well. The stained cells were then imaged using an EVOS fluorescence
microscope (EVOS FL color, Life Technologies, Thermo Fisher Scientific,
UK).
Statistical Analysis
Two-way ANOVA with Tukey’s
multiple comparison test was used for statistical analysis from the
GraphPad Prism 8 software package from GraphPad Software, Inc., USA.
All data were expressed as mean ± standard deviation (SD), and p < 0.05 was considered statistically significant.
Results and Discussion
Synthesis and Characterization of AIS-2MPA
QDs
One
of the major hurdles in nanotechnology is the stability of nanoparticles.[58] 2MPA was shown to be a good coating material
because it dramatically increases the stability of the nanoparticles
and enhances the luminescence intensity.[29,59] Hence, anionic AgInS2 (AIS) QDs were synthesized under
aqueous conditions in the presence of 2MPA at RT at different Ag/In/S/2MPA
ratios, and their influence on the optical properties and stability
of QDs was determined (Table , Figure , Figure S1). All the emission peaks were quite
broad, with FWHM between 79 and 219 nm (Table ). Such a broad emission profile (Figure ) coupled with the
featureless absorbance spectrum (Figure S1) of such ternary QDs is attributed not only to size distribution
but also to compositional inhomogeneity of the crystals, structural
defects, and related mid-gap energy states, resulting in not only
band-edge but also donor–acceptor recombination and trap state
emissions.[7,19] In general, these AIS-2MPA QDs show a major
peak maximum around 630–660 nm and a shoulder at a longer wavelength
of 705–715 nm. This is in line with the reported emission profiles
for the AIS QDs and the explanation mentioned above about radiative
events.[7,19,60] Bandgap energy
determination of AIS is relatively tricky due to the uncertainty in
electron-hole mass values and long absorbance tail.[61] The bandgaps of these QDs calculated from the absorption
spectra by replotting the data in the coordinates of the Tauc equation
were found as 2.10–2.34 eV (Figure S2, Table ). These
values agree well with the Eg reported
for AIS.[62,63] On the other hand, when these values are
evaluated, an inevitable error originating from the long absorbance
tails masking the exact position of the band edge should be taken
into account.[62,64] Such long absorbance tails are
attributed to the localized defect states within the crystals providing
the sub-band states and hence the long absorbance tails and broad
emissions.[64] The absorption tail is called
the Urbach tail and is associated with the Urbach energy (Eu) that can be calculated using the following:where α is the absorption coefficient, E is
the photon energy (hν), and Eu is the Urbach energy. By plotting the ln(α)
against E, the Urbach energy can be calculated from
the slope of the linear fit (Figure S3a–e).[63] The Urbach energies of these AIS
QDs are between 137 and 172 meV and show an increasing trend with
the decreasing emission maxima, suggesting more disorder in the crystals
as the size decreases. These Eg and Urbach
energies agree with the values reported in the literature for the
different anionic AIS QDs.[22,64]
Figure 1
(a) PL spectra of the
AIS-2MPA QDs prepared with a constant molar
ratio of Ag/In 1/4, cations/coating 1/5, and different molar ratios
of Ag/S. (b) PL spectra of the AIS-2MPA QDs prepared with a constant
molar ratio of Ag/S 1/10, cations/coating 1/5, and different molar
ratios of Ag/In. (c) PL spectra of all the AIS-2MPA QDs prepared at
different conditions. (d) XRD (AIS JCPDS: 25-1328), (e) FTIR, (f)
Ag 3d, (g) In 3d, and (h) S 2p XPS spectra of the AIS-2MPA-3 QDs.
(a) PL spectra of the
AIS-2MPA QDs prepared with a constant molar
ratio of Ag/In 1/4, cations/coating 1/5, and different molar ratios
of Ag/S. (b) PL spectra of the AIS-2MPA QDs prepared with a constant
molar ratio of Ag/S 1/10, cations/coating 1/5, and different molar
ratios of Ag/In. (c) PL spectra of all the AIS-2MPA QDs prepared at
different conditions. (d) XRD (AIS JCPDS: 25-1328), (e) FTIR, (f)
Ag 3d, (g) In 3d, and (h) S 2p XPS spectra of the AIS-2MPA-3 QDs.
Influence of the Experimental Variables on
the Optical Properties
of AIS-2MPA QDs
Influence of the Ag/S Molar Ratio
To evaluate the effect
of the Ag/S ratio (1/1.25, 1/2.5, and 1/10) on the optical properties
of the produced QDs, varying amounts of the sulfur precursor were
used while the other variables were fixed (Ag/In: 1/4, cations/coating:
1/5) (Table ). Increasing
the sulfur precursor blue-shifted the major peak maxima from 701 to
634 nm with an accompanying blue shift in the absorbance spectra (Figure a, Figure S4a).These three recipes have indeed cation/S
ratios of 0.5, 2, and 4 for AIS-2MPA-1, AIS-2MPA-2, and AIS-2MPA-4,
respectively. So, in a way, as the Ag/S ratio decreased, the cation/S
ratio also decreased, and a resultant blue shift in emission maxima
was observed. This was probably due to an increasing stoichiometric
imbalance as the formulations switched from cation-rich to S-rich,
thereby reducing the crystal size. The smaller crystals were also
accompanied by a stronger emission and a higher QY, which may be partially
due to better passivation of the smaller crystals, lower degree of
aggregation, and fewer crystal defects.These observations are
in line with the GSH-coated ZAIS reported
by Deng et al.[7] and the PEI-coated AIS
reported by Raevskaya et al.[25]Eg decreased and Eu increased with the decreasing Ag/S ratio. The relatively large Eus and broad long-wavelength emission tail may
support the significant emissions from the trap states. Here, a Ag/S
ratio of 1/2.5 yielded the highest PL intensity. However, due to the
lack of colloidal stability during the washing step, they could not
be studied further. Because the QDs produced at a Ag/S molar ratio
of 1/10 were the most luminescent and the stable QDs, this ratio was
kept fixed to study the influence of the In/S ratio on the QD properties.
Influence of the Ag/In Molar Ratio
To further investigate
the opportunity to tune the optical properties of the AIS-2MPA QDs,
the ratio of Ag/S was fixed to 1/10, whereas the Ag/In ratio was varied
as 1/2, 1/4, and 1/10 (molar ratio of cations/coating: 1/5) (Figure b, Figure S4b). Although the emission peaks were broad again,
increasing the In content (decreasing Ag/In ratio) caused a slight
blue shift in the emission maxima from 649 to 630 nm. This trend is
in agreement with the earlier reports.[19,23] Based on the
HOMO–LUMO analysis of Tsuji et al., as the Ag content decreases,
the hybrid orbitals of In5s and S3p become the major HOMO, instead
of the hybrid orbitals of S 3p and Ag 4d, which increases the bandgap
causing a blue shift in the emission.[65]The Ag/In ratio substantially impacted the emission intensity,
and the strongest emission was achieved at the highest Ag/In ratio
of 1/10. The in-excess formulation is preferred due to the reactivity
difference of Ag+ (soft acid) and In3+ (hard
acid) with sulfide ( soft base) in the formation of ternary structures.[66,67] Besides, it was suggested that higher QYs of In-rich recipes are
correlated with an increased order in the In sublattices and reduction
of intrinsic defects.[68]A Ag/In ratio
of 10 also corresponded to the cations/S ratio of
1.1 (AIS-2MPA-3), whereas others had a ratio of 0.5 (AIS-2MPA-1) and
0.3 (AIS-2MPA-5). Thus, this set’s cation-rich formulation
may provide a better surface binding of the 2MPA and eliminate the
surface defects. Indeed, when the emission profiles of these three
QDs are examined, relatively strong intensities of the long-wavelength
emission peaks are noticed, whereas AIS-2MPA-3 has a strong emission
peak at 630 nm with quite a weak contribution of the long-wavelength
emission (Figure b).
This may be due to the reduced defects and related emissions that
appear as the long-wavelength peak in these ternary QDs.[19]To follow the growth of the particles,
aliquots were taken from
the reaction mixture at discrete time points, and their optical properties
were examined, as it is believed that crystal growth kinetics play
an important role in tuning the particle size and emission.[69] Prolonged reaction times could influence crystallinity,
change the crystal composition, and promote particle growth via the
Ostwald ripening process.[19,70] However, at extended
reaction times, oxidation of the ligands, agglomeration of the nanoparticles,
and the formation of defects may decrease the luminescence intensity.[71]Figure S1 shows the
time-dependent changes in the emission and absorbance profile of the
AIS-2MPA QDs. Nearly no change in the absorption onset was observed
with the increase of growth time, suggesting no dramatic change in
the size. The reaction duration mainly influenced the emission intensity
rather than the peak maxima, suggesting that particle surfaces were
well passivated but possibly underwent surface reconstruction.The photoluminescence QYs of the AIS-2MPA-1 and AIS-2MPA-3 QDs
are about 10 and 19% (Table ). Hence, the best recipe for the synthesis of the colloidally
stable and highly luminescence anionic AIS-2MPA has a molar ratio
of Ag/In/S 1/10/10. Therefore, a new batch of AIS-2MPA-3 was synthesized
and used in all the in vitro studies with emission maxima at 634 nm,
5.2 nm (number-based hydrodynamic size) diameter, and −37.5
mV zeta potential (Table S1).
Structural
Characterization of AIS-2MPA QDs
Structural
characterization of AIS-2MPA was performed using the AIS-2MPA-3 QDs.
The broad diffraction peaks detected via XRD analysis are attributed
to tetragonal AIS QDs (Figure d).[19] The FTIR spectrum of this
QD provided information about the coating molecule (Figure e). The disappearance of the
S–H stretching band, which would be between 2500 and 2540 cm–1, indicates the binding of 2MPA to the AIS core by
its thiol.[10,59] The stretching band of the C=O
observed at 1567 cm–1 is consistent with the carboxylic
acid interacting with the crystal surface. The broad absorption band
at 3300 cm–1 can be attributed to the OH group,
and the band at 1395 cm–1 corresponds to the C–O
stretching vibrations of 2MPA bound to the AIS crystals, respectively.[10,72] XPS analysis provided further information about the composition
(Figure f–h).
The Ag 3d core level peaks at binding energies (BE) of 367.10 eV (3d5/2)
and 373.14 eV (3d3/2) fit well to the Ag+. The In 3d peaks
at BE of 444.06 eV (3d5/2) and 451.58 eV (3d3/2) fit to the In3+ of AIS. The doublet at BE of 160.51 and 161.81 eV fits to
the 2p3/2 and 2p1/2 of Ag–S, respectively. The other doublet
at 161.30 and 162.71 eV belongs to the S of 2MPA.[7,57] According
to the XPS data, the Ag/In and Ag/S ratios were 1/7.5 and 1/11.5,
which were consistent with the Ag/In ratio of 1/7 and Ag/S ratio of
1/12 determined by ICP. TGA analysis performed on the AIS-2MPA-3 QD
indicates 62.8% organic content (Figure S4d). The TEM images of these QDs indicate small particles with an average
diameter of 5.85 ± 0.74 nm (Figure S4e–f). EDS analysis shows colocalization of Ag and In and a broader distribution
of S, which is in the core and the coating (Figure S4g).
Synthesis and Characterization of AIS-PEI/2MPA
QDs
In developing the PEI-coated Ag2S, we have
previously
shown that PEI coating does not produce luminescent particles, but
PEI/2MPA does.[73] The most stable and luminescent
Ag2S-PEI/2MPA QDs (AS-PEI/2MPA) were synthesized at pH
9 at a Ag/coating molar ratio of 1/5 and PEI/2MPA ratio of 4/1.[73] Based on this knowledge, cationic AIS QDs were
prepared with PEI/2MPA coating in water with slow addition of sulfide
to the salt mixtures[7,9] The introduction of Na2S into the solution containing Ag/In-PEI/2MPA produced a cloudy solution
with yellow to brown coloration depending on the molar ratio of the
components. The emission peak profiles of the AIS-PEI/2MPA QDs resemble
those observed for AIS-2MPA: broad emission peaks with a long wavelength
shoulder or tail due to various radiative coupling events involving
the trap states and donor–acceptor pair recombination (Figure S6). With the different recipes wherein
the stoichiometry of Ag/In/S was changed, AIS-PEI/2MPA QDs emitting
in the red-NIR region with an emission peak maxima between 774 and
617 nm were obtained (Table , Figure , Figure S7a–g). The bandgap energies of
these cationic AIS QDs were calculated between 2.02 and 2.74 eV from
the Tauc plots (Figure S8) and Urbach energies
between 138 and 168 meV (Figure S9). Indeed,
these energies agree with the only reported PEI-coated AIS.[25]
Figure 2
(a) PL spectra of the AIS-PEI/2MPA QDs prepared with a
constant
molar ratio of Ag/In 1/4, cations/coating 1/5, and different molar
ratios of Ag/S. (b) PL spectra of the AIS-PEI/2MPA QDs prepared with
a constant molar ratio of Ag/S 1/10, cations/coating 1/5, and different
molar ratios of Ag/In. (c) PL spectra of all AIS-PEI/2MPA QDs prepared
at different conditions. (d) XRD (AIS JCPDS: 25-1328), (e) FTIR, (f)
Ag 3d, (g) In 3d, and (h) S 2p XPS spectra of the AIS-PEI/2MPA-1 QDs.
(a) PL spectra of the AIS-PEI/2MPA QDs prepared with a
constant
molar ratio of Ag/In 1/4, cations/coating 1/5, and different molar
ratios of Ag/S. (b) PL spectra of the AIS-PEI/2MPA QDs prepared with
a constant molar ratio of Ag/S 1/10, cations/coating 1/5, and different
molar ratios of Ag/In. (c) PL spectra of all AIS-PEI/2MPA QDs prepared
at different conditions. (d) XRD (AIS JCPDS: 25-1328), (e) FTIR, (f)
Ag 3d, (g) In 3d, and (h) S 2p XPS spectra of the AIS-PEI/2MPA-1 QDs.The colloidal AIS-PEI/2MPA
QDs synthesized with different Ag/S ratios at a constant Ag/In ratio
of 1/4 and cations/coating ratio of 1/5 exhibited emission peaks with
a maximum between 618 and 655 nm (AIS-PEI/2MPA-1, 3, and 6) with no
significant tuning of the peak position. The dramatic difference in
the PL intensity indicates stronger emission with the decreasing Ag/S
ratio reaching its maximum at a Ag/S ratio of 1/10 (Figure a). Thus, this ratio is chosen
as the optimum Ag/S ratio for the following experiments. Although
there is no clear correlation between the PL peak maxima, bandgap
energy, Urbach energy, and the Ag/S ratio (Figures S8, S9, and S10a), in general, bandgap widening with the decreasing
Ag/S ratio was observed within this series (like the same trend in
the AIS-2MPA QDs).[65,66] These three recipes are all cation-rich,
but excess Ag may be another source of defects increasing the Eu.[25]
Influence
of the Ag/In Molar Ratio
At a fixed Ag/S
ratio of 1/10, the Ag/In ratio was varied from 1/0.25 to 1/10 (AIS-PEI/2MPA-1,
2, 4, and 7) (Table , Figure b) while
keeping the other reaction conditions constant. A blue-shifted absorbance
onset and emission peak maxima (from 774 to 617 nm) with the decreasing
Ag/In molar ratio (increasing cation/S ratio) was observed as in AIS-2MPA
(Figure S10b). The PL and UV–vis
spectra of all QDs produced with the varied reaction variables are
shown in Figure c
and Figure S10c, respectively. According
to Hu et al.,[71] the blue-shifted emission
with the decreasing content of Ag in the AIS QDs may originate from
the defect-related recombinations instead of the transition between
the quantized energy levels in the conduction and valence bands due
to their large Stokes shift. Here, Eg increased
from 2.02 to 2.7 eV with the decreasing Ag/In ratio, which supports
blue-shifted spectra.[28,65] The Eu increased from 138 to 167 meV with the increase in the Ag/In ratio
(Table ), indicating
the increasing structural defects and disorders within the crystal
(Figure S9).[58] This indeed may indicate more crystal distortions and defects in
the S-rich formulations. Overall, the most stable and luminescent
cationic QDs are synthesized with a molar ratio of Ag/In/S 1/10/10
(AIS-PEI/2MPA-1) with ca. 20% QY, which is again a cation-rich formulation.
These cationic QDs with emission maxima at 617 nm, zeta potential
of 10.67 mV, and hydrodynamic size of 7.66/27.91 nm (number based/intensity-based
average) were used for further characterizations and in vitro studies.
This QD had the highest QY with a weak long wavelength tail in the
emission spectra suggesting fewer defects in the crystals, which may
be at least partially due to the cation-rich formulation that the
ligands can better stabilize. Here, it is important to point out that
the ultra-small cationic QDs (based on the hydrodynamic size) are
obtained with such QY in a single step reaction at RT using the PEI/2MPA
mixture. RT synthesis prevents S-release from mercaptoacids, and in
the PEI coating, contribution of 2MPA provides strong surface binding
and reduces the defects compared to the use of only PEI.One
example of cationic AIS QDs in the literature uses only PEI in reflux
conditions producing 100 nm aggregates with 4–5 nm crystal
size and achieved 20% QY (with respect to anthracene) only after 2
h of heat treatment at 100 °C.[25] The
other example to the pure PEI (10 kDa)-coated AIS QDs had a small
hydrodynamic size and 32% QY but used a pressure cooker (120 °C)
and did not report any long-term colloidal or luminescence stability.[22] Both had maximum emission below 600 nm. These
examples clearly indicate the advantage of using a mixed coating and
its utility in tuning size emission and imparting strong emission
in an RT reaction.
Structural Characterization of AIS-PEI/2MPA
QDs
The
XRD pattern of AIS-PEI/2MPA-1 consists of the characteristic peaks
of the tetragonal and orthorhombic AIS structure (Figure d).[74] The FTIR spectrum of the AIS-PEI/2MPA-1 (Figure e) indicated the presence of the stretching
vibrations at 1585 and 1405 cm–1, which are generally
assigned to the binding mode of carboxylates to a surface or to a
cation. The bands at 3387 and 2850–2960 cm–1 correspond to the stretching modes of the N–H and C–H
bonds of PEI, respectively.[11] The absence
of the thiol peak in the range of 2500–2550 cm–1 confirms the covalent conjugation of the inorganic core to 2MPA
via its thiol.[72] XPS analysis provided
further information about the AIS-PEI/2MPA-1 QDs. The XPS spectra
obtained in Figure f–h confirmed the presence of the following elements: Ag 3d5/2
and 3d3/2 at BE of 372.92 and 336.94 eV and In 3d5/2 and 3d3/2 at
BE of 451.38 and 443.79 eV. The two doublets were observed for S.
BE of 160.22 (2p3/2)–162.57 eV (2p1/2) correspond to the core
S, and 160.93 (2p3/2)–162.35 eV (2p1/2) corresponds to the
bound S of 2MPA. These are consistent with the reported values for
the AIS QDs and those observed for AIS-2MPA (Figure f–h).[74] The N 1s region could be fitted to the two peaks at 398.20 and 401.12
eV, corresponding to the tertiary, secondary, and primary amines of
PEI (Figure S10d). The high binding energy
N 1s peak indicates primary amine binding to the crystal surface.[73] The atomic ratio of the elements calculated
from the area under each curve indicated a Ag/In/S ratio of 1/9/10,
which is consistent with the theoretical ratio of 1/10/10. This ratio
also agrees with the atomic ratio measured by ICP as Ag/In/S = 1/8.8/10.8.
TGA analysis performed on the AIS-PEI/2MPA-1 QD indicates 58.6% organic
content (Figure S10e). The TEM images of
these QDs also indicate small particles with an average diameter of
6.1 ± 1.7 nm (Figure S10f–g).
EDS analysis shows colocalized Ag and In with broader distribution
of S, which is also coming from the 2MPA component of the mixed coating
(Figure S10h).
Colloidal Stability of
the QDs
The shelf life of the
nanoparticles is critical for any practical application. Generally,
the PL intensity of QDs decreases over time due to the desorption
of the ligands and/or oxidation, which may also cause an increase
in the hydrodynamic size and precipitation.[73] The emission and absorbance characteristics (PL and UV–vis
spectra), hydrodynamic size, and zeta potential of the most luminescent
QDs over a period of 3 months were tracked to determine the stability
of the colloidal anionic and cationic AIS produced here (Figure and Table S1). The colloidal QDs were stored at 4
°C after being washed. The emission intensity of both QDs increased
with time, similar to Ag2S-2MPA, which was reported before
(Figure a,e).[27] To better understand the time dependence of
PL intensity, the kinetics of the photogenerated charge carriers were
studied using the time-resolved PL spectra of these QDs.
Figure 3
(a,e) PL spectra
and (b,f) normalized UV–vis spectra and
(c,g) PL lifetime of the AIS-2MPA-3 and AIS-PEI/2MPA-1 QDs at the
1st day and 3rd month of their synthesis, respectively. The inset
shows the fit parameters of the decay curves. (d,h) Colloidal stability
of the AIS-2MPA-3 and AIS-PEI/2MPA-1 QDs at different time points
following its synthesis.
(a,e) PL spectra
and (b,f) normalized UV–vis spectra and
(c,g) PL lifetime of the AIS-2MPA-3 and AIS-PEI/2MPA-1 QDs at the
1st day and 3rd month of their synthesis, respectively. The inset
shows the fit parameters of the decay curves. (d,h) Colloidal stability
of the AIS-2MPA-3 and AIS-PEI/2MPA-1 QDs at different time points
following its synthesis.All the decay profiles
were fitted according to the function of
[I(t) = A1exp(−t/τ1) + A2exp(−t/τ2)],
where τ1 and τ2 are the decay times
and A1 and A2 are the fractional contributions of the two components.[6] Generally, the fast component τ1 represents the bandgap recombination and the slow component, τ2 is related to the defect-related radiative recombination
of the carriers.[7] They were also suggested
as high energy, intrinsic defect-related, donor–acceptor coupling
versus low energy, surface effect-related emissions for the AIS QDs.[63] For these AIS QDs, both τ1 (18–25
ns) and τ2 (161–165 ns) are relatively shorter
than most AIS reported in the literature.[25,74] The average lifetimes calculated from <τ> = (A1τ12 + A2τ22)/(A1τ1 + A2τ2) are also relatively shorter than the AIS QDs, which also
have lower
QYs than the ones produced here (inset table Figure c,g).[6] The contribution
of τ1, which was around 24.9 and 18.6 ns, was 9 and
13% for the AIS-2MPA-3 and AIS-PEI/2MPA-1 QDs, respectively. After
3 months of storage, τ1 and τ2 became
longer, 30.4 and 22.6 ns, with an increased contribution, which is
about 11.7 and 16.5% for the anionic and cationic AIS QDs, respectively.
The ratio of A2/A1 decreased from 9.9 to 7.6 in AIS-2MPA-3 and from 6.8 to 5
in the AIS-PEI/2MPA-1 QDs after 3 months, indicating more contribution
of the band edge and/or intrinsic defects than the surface defects
with time.[23] This was accompanied by a
slight blue shift in the emission maxima from 632 to 612 nm for the
anionic QDs and from 617 to 593 nm for the cationic AIS QDs (Table S1). The enhanced contribution of fast
component, usually accompanied by a blue shift in the emission maxima
of AIS or ZAIS QDs, indicates a lesser contribution of or say fewer
surface defects.[25,60,63] The hydrodynamic size of the QDs showed a slight increase after
3 months (Table S1). However, the high
surface charge of both the AIS-2MPA-3 (−44.56 eV) and AIS-PEI/2MPA-1
QDs (11.75 eV) prevented any significant aggregation/precipitation,
and they have maintained small hydrodynamic sizes that may be desired
for any biological application (Table S1).In summary, we can say that the particles are colloidally
stable
and no aggregation, precipitation, or quenching was observed after
3 months (Figure d,h),
but instead, an enhancement in the luminescence intensity was detected
(Figure a,e). Hence,
they are very suitable for exploitation in in vitro studies.
Electrostatic
Loading of ALA to AIS-2MPA-3 and AIS-PEI/2MPA-1
ALA has one
carboxylic acid and one primary amine group with pKa values of 4.05 and 8.9, respectively. ALA
should be zwitterionic at pH 7.2–7.4, and the electrostatic
interaction between the −COO– group of the
AIS-2MPA-3 QDs and the −NH3+ group of
ALA can allow the electrostatic loading of ALA to the anionic QDs.
Two compositions were prepared with 30 and 50 mol % ALA loading (with
respect to the 2MPA content of the QD) to AIS-2MPA-3. This increased
the intensity-based hydrodynamic size of the AIS-2MPA-3 QDs from 38
to 62 and 50 nm, respectively, in HEPES buffer (pH = 7.2) (Table S2). This indicates some aggregation; however,
the number-based size average does not indicate a dramatic aggregation
(5.2 nm versus 5.7–5.9 nm). The zeta potential of the QDs changed
slightly from −42 mV to −43 and −44 mV for 30
and 50% ALA loadings, respectively (Table S2). Although the carboxylate groups of the QDs are consumed by the
NH3+ groups of ALA, the −COO– groups of ALA reside on the periphery after binding; therefore,
the zeta potential did not change much. In the AIS-PEI/2MPA-1 QDs,
at pH 7.2 in HEPES buffer, the −NH3+ groups
of QDs are electrostatically bound to the −COO– groups of ALA. This increased the charge of the AIS-PEI/2MPA-1-30%ALA
and AIS-PEI/2MPA-1-50%ALA QDs from ca. 11 to 12 and 16 mV, respectively
(Table S2). This prevented aggregation,
and the hydrodynamic size stayed around 27–33 nm with a reduced
size distribution (Table S2). Again, the
number-based average hydrodynamic size increased slightly from 7.6
to 9–10 nm with the ALA loading (Table S2). Overall, after the ALA loading, both QDs maintained small
hydrodynamic sizes and their original charge character as desired
for this study.ITC has been used further to study the interaction
between ALA and the QDs. Titration of QDs at pH 7.2 for AIS-2MAP-3
and AIS-PEI/2MAP-1 with 50 mol % ALA dissolved in HEPES buffer created
an exotherm, which is an indication of binding (Figure S11a,b). The exotherm regularly decreased with the
addition of ALA and reached almost to a constant value at the last
injection. This suggests that ALA fully binds to both cationic and
anionic AIS QDs at the studied doses. Yet, the binding exotherm is
much stronger in the cationic AIS QDs, indicating stronger binding
(Figure S11a,b).The best drug delivery vehicles
are supposed to bind strongly to the drug at the physiological pH
and then release it effectively at the diseased site.[75] Because ALA is loaded to the QDs via the electrostatic
interaction, the pH changes should affect its release. AIS-2MPA-3-50%ALA
and AIS-PEI/2MPA-1-50%ALA were incubated in PBS at acidic and neutral
pH (5.5 and 7.4) for 40 h at 37 °C. Protonation of the carboxylic
acids in acidic pH would weaken the electrostatic interaction between
the anionic QD and ALA, causing its release. In the cationic QDs with
the PEI content, protonation of amines and the 2MPA component will
also weaken the interactions as ALA may have started to protonate
as well. In the in vitro studies, the effective release of the anionic
cargo from the PEI-containing delivery vehicles is also associated
with the proton-sponge effect. Here, both QDs kept the release of
ALA ≤15% at pH 7.4 in 24–40 h. A small burst release
around 10% was followed by a sustained release profile in acidic media.
In general, the release from the cationic QDs was slightly faster,
reaching 30% in 5 h and a maximum value of 80% in 25 h. The ALA release
from the anionic QD was about 20% in 5 h and 72% after 31 h in acidic
pH. The enhanced ALA release in the acidic media should facilitate
the therapeutic efficacy of the conjugates under the acidic tumor
microenvironment in vivo. The emission intensity of the QDs after
the 40 h ALA release at pH 5.5 showed only 20–30% reduction
(Figure S11e–h), suggesting that
appreciable stability of the QDs can be attained in a tumor microenvironment
or acidic intracellular compartment. Xu et al. have demonstrated that
ALA conjugated to gold nanorods via hydrazone linkage, which hydrolyzes
under an acidic tumor environment, release 71% of ALA at pH 5 in 24
h and only 6% of ALA at neutral pH.[80] In
a study conducted by our group, the ALA release from the electrostatic-loaded
ALA to anionic Ag2S QDs was reported ∼50% after
24 h in acidic media, whereas it was ∼25% at neutral pH.[76] It is quite promising to see similar pH selectivity
in release with the simply electrostatically loaded ALA to our QDs.
The ALA release was much less in amount with poor pH dependence from
the self-assembled polysaccharide-based nanocomplexes reported by
Wang et al., which trapped ALA non-covalently. They reported 15 and
20% release of ALA in 5 h and 30% and 50% after 24 h at pH 7.4 and
pH 5.5, respectively.[48] Here, both the
cationic and anionic QDs effectively protect ALA under physiological
pH, which would minimize the leakage during circulation, but release
the prodrug effectively at the endosomal/lysosomal pH, nominating
these QDs as promising candidates for successful ALA delivery. The
strong luminescence of the AIS QDs would also provide image-guided
therapy of the are occupied by the nanoparticles and hence ALA, which
would aid the operator to decide when to irradiate and highlight the
sensitized region for the high level of locality in the treatment,
which is undoubtedly very desirable for the improved therapeutic outcome
with reduced side effects.
Evaluation of In Vitro Dark Cytotoxicity
of the QDs
Cytotoxicity of the AIS-2MPA-3 and AIS-PEI/2MPA-1
QDs and their ALA
conjugates on various tumor cells was determined using the 2D cell
culture of the HT29, HeLa, SW480, and HCT116 cell lines by the MTT
assay (Figure S12). The QD doses were based
on the total cation concentration of each QD determined by ICP-MS
and studied in the range of 0.25–100 μg/mL. The AIS-2MPA-3
QDs did not show any significant cytotoxicity in this range after
48 h incubation (Figure S12a–d).
The AIS-PEI/2MPA-1 QDs significantly impaired the cell viability of
all tested cell lines at cation concentrations above 2 μg/mL
(Figure S12e–h). PEI has a dose-
and molecular weight-dependent toxicity due to its cationic nature,
which is suppressed significantly by adsorption on the QD surface.[73] Hence, the cationic nanoparticles are expected
to be more toxic. Free ALA did not show any substantial cytotoxicity
in either of the tested cell lines up to 0.69 mM, the highest concentration
delivered at 100 μg/mL cation concentration. Although the cell
viability slightly decreased when exposed to the ALA-loaded cationic
QDs compared to the free QDs, ALA association with QDs did not lead
to a dramatic difference between different formulations. The influence
of these QDs on the viability of healthy colorectal cells was also
tested. There was no loss in the viability of the CCD841 cells that
were exposed to free ALA, AIS-2MPA-3 QDs (up to 200 μg/mL [cations]),
or ALA-loaded AIS-2MPA-3 QDs (Figure S13a). In the AIS-PEI/2MPA-1 QDs and its ALA-loaded formulations, a significant
drop in the cell viability was observed at 10 μg/mL cation concentration,
which is mostly due to the cationic nature of the QDs because ALA
did not cause any reduction in cell viability (Figure S13b).
In Vitro Cell Uptake and Optical Detection
HT29, HeLa,
SW480, and HCT116 cells treated with 2 μg/mL [cation] of AIS-2MPA-3
and AIS-PEI/2MPA-1 QDs for 24 h exhibited intense intracellular optical
signals, indicating effective internalization of both QDs to each
cell line (Figure a–d). The intensity and clarity of the intracellular signal
support the potential of these QDs for optical–medical imaging.
There seems to be more luminescence in the cells treated with the
cationic QDs. Hence, to quantify the uptake of QDs by these cell lines,
the concentration of Ag and In in the QD-treated cells was determined
by ICP-MS. After 24 h incubation with QDs (2 μg/mL), about 20–25%
of the AIS-PEI/2MPA-1 and 10–15% of the AIS-2MPA-3 QDs were
internalized by the different cell lines according to the ICP-MS analysis
of the lysed cells with no significant difference between different
cell lines (Figure e). In addition to the more toxic nature of PEI than 2MPA, this higher
uptake of the cationic QDs may also contribute to the higher toxicity
of the AIS-PEI/2MPA-1 QDs.
Figure 4
Cellular localization of the control cells,
AIS-PEI/2MPA-1, and
AIS-2MPA-3 QDs by (a) HT29, (b) HeLa, (c) SW480, and (d) HCT116 cells.
The samples at 2 μg/mL cation concentration were incubated with
cells for 24 h in 2D culture. Red: luminescence from the QDs (excitation/emission:488/580–780
nm), blue: nuclear stain. (e) Intracellular quantification of AIS-PEI/2MPA-1
and AIS-2MPA-3 QDs in HeLa, SW480, HT29, and HCT116 cell lines in
2D culture. Measurements were done by an ICP-MS instrument. The samples
at 2 μg/mL cation concentration were incubated with cells for
24 h. The data are expressed as mean ± S.D. using two-way ANOVA
with Tukey’s multiple comparison test (n =
3), (p < 0.05).
Cellular localization of the control cells,
AIS-PEI/2MPA-1, and
AIS-2MPA-3 QDs by (a) HT29, (b) HeLa, (c) SW480, and (d) HCT116 cells.
The samples at 2 μg/mL cation concentration were incubated with
cells for 24 h in 2D culture. Red: luminescence from the QDs (excitation/emission:488/580–780
nm), blue: nuclear stain. (e) Intracellular quantification of AIS-PEI/2MPA-1
and AIS-2MPA-3 QDs in HeLa, SW480, HT29, and HCT116 cell lines in
2D culture. Measurements were done by an ICP-MS instrument. The samples
at 2 μg/mL cation concentration were incubated with cells for
24 h. The data are expressed as mean ± S.D. using two-way ANOVA
with Tukey’s multiple comparison test (n =
3), (p < 0.05).Fluorescence microscopy was also conducted on the 3D spheroids
of HT29 and SW480 cells with AIS-PEI/2MPA-1 (2 μg/mL) and AIS-2MPA-3
QDs (2 and 50 μg/mL) and their ALA-loaded formulations (Figure S14a,b). Both QDs showed strong luminescence,
and in the anionic ones, the optical signal seemed to be stronger
as the concentration increased. The ALA-loaded versions seem to provide
more signal, especially in SW480, probably due to PpIX generation
with luminescence at around the same wavelengths as these AIS QDs.
Overall, the bright red fluorescence observed in the 3D matrix originates
from the embedded cells rather than the collagen matrix. This strong
AIS-based intracellular luminesce observed within the 3D matrix further
supports the candidacy of these QDs for optical imaging and/or utilization
of such nanoparticles for image-guided therapy.
In Vitro PDT
Studies
ALA can act as a prodrug of a
strong photosensitizer, PpIX, which produces highly toxic ROS upon
irradiation, causing apoptosis/necrosis. After the internalization
of the ALA conjugates by the cells, ALA was converted to PpIX via
the heme-synthesis pathway.[77] Therefore,
delivery of ALA into the cells in a therapeutic dose, its release,
and its intracellular conversion to PpIX in the cancer cells are crucial
steps for effective PDT. The fluorescence of PpIX at 635 nm can be
used to determine the intracellular PpIX amount. However, because
QDs have absorbance at an excitation wavelength of 420 nm and luminescence
at the same region with PpIX, it interfered with the measurements
(Figure S15). Yet, an indication of higher
PpIX generation with the QD-loaded ALA was observed in addition to
a slight dose and cell type dependence mostly at high concentrations.
The differences between the generated PpIX in the cell lines are due
to the various ALA metabolisms and conversion of ALA to PpIX by different
mitochondrial enzymes.[76]In vitro
PDT studies were performed on the 2D and 3D cell cultures using blue
light (420 nm, 7 mW/cm2) for 5 min. Because MTT is not
suitable to check viability in 3D cell cultures, Alamar blue was used
to determine the viability of cells before and after PDT (Figure ). The viabilities
of the 2D-cell cultures after PDT were also tested with the MTT assay
(Figure S16). All doses were based on ALA
in Figure because
it is critical to compare the phototoxicity of free ALA versus QD-delivered
ALA. The corresponding QD concentrations are given in Table S2. All PDT studies were performed on two
colorectal cancer cell lines: SW480 and HT29.
Figure 5
Viability of (a,b) HT29
and (c), (d) SW480 cells treated with AIS-2MPA-3,
AIS-2MPA-3-30%ALA, and AIS-2MPA-3-50%ALA QDs and (e,f) HT29 and (g,h)
SW480 cells treated with AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and
AIS-PEI/2MPA-1-50%ALA QDs after 24 h incubation with and without PDT
measured by Alamar blue compared to the untreated cells. Viability
of 0.35 mM ALA of AIS-2MPA-3, AIS-2MPA-3-30%ALA, and AIS-2MPA-3-50%ALA
QDs on (i) HT29 and (j) SW480 3D-spheroid models and 0.015 mM ALA
of AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and AIS-PEI/2MPA-1-50%ALA
on (k) HT29 and (l) SW480 3D-spheroid models treated with QDs and
illuminated at 420 nm blue light for 5 min. PDT control indicated
cells treated only with 420 nm irradiation for 5 min. The data are
expressed as mean ± S.D. using two-way ANOVA with Tukey’s
multiple comparison test (n = 3), (p < 0.05).
Viability of (a,b) HT29
and (c), (d) SW480 cells treated with AIS-2MPA-3,
AIS-2MPA-3-30%ALA, and AIS-2MPA-3-50%ALA QDs and (e,f) HT29 and (g,h)
SW480 cells treated with AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and
AIS-PEI/2MPA-1-50%ALA QDs after 24 h incubation with and without PDT
measured by Alamar blue compared to the untreated cells. Viability
of 0.35 mM ALA of AIS-2MPA-3, AIS-2MPA-3-30%ALA, and AIS-2MPA-3-50%ALA
QDs on (i) HT29 and (j) SW480 3D-spheroid models and 0.015 mM ALA
of AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and AIS-PEI/2MPA-1-50%ALA
on (k) HT29 and (l) SW480 3D-spheroid models treated with QDs and
illuminated at 420 nm blue light for 5 min. PDT control indicated
cells treated only with 420 nm irradiation for 5 min. The data are
expressed as mean ± S.D. using two-way ANOVA with Tukey’s
multiple comparison test (n = 3), (p < 0.05).Anionic AIS-2MPA-3 and its ALA-loaded
versions showed no dark toxicity
in the studied range (Figure a,c). ALA created effective toxicity upon irradiation only
at the highest dose, 0.35 mM in the HT29 cell line, and at and above
0.17 mM in the SW480 cell line. However, the ALA-loaded AIS-2MPA-3
QDs induced greater phototoxicity in a dose- and ALA loading-dependent
manner. The viability of the HT29 cells dropped to ∼40% (30%
ALA loading) and ∼30% (50% ALA loading) at 0.35 mM ALA, respectively,
whereas free ALA provided 75% viability at this dose. The effect was
more dramatic on the SW480 cells with ∼40% (30% ALA loading)
and ∼20% (50% ALA loading) viability, whereas free ALA provided
∼70% viability at 0.35 mM ALA. Because no phototoxicity was
detected in the cells treated with AIS-2MPA-3, enhanced phototoxicity
should indicate better ALA-PDT when delivered with these nanoparticles
(Figure b,d).AIS-2MPA-3-30%ALA provided IC50 at 0.29 mM and 0.25 mM in HT29
and SW480 cells. This was improved by using AIS-2MPA-3-50%ALA QDs:
IC50 was 0.11 and 0.09 mM for HT29 and SW480 cells, respectively.
Our recent study has shown about 60 and 40% reduction in viability
of SW480 and HT29 cell lines treated with ALA-loaded (0.35 mM [ALA])
anionic Ag2S QDs after 5 min irradiation at 420 nm.[76] The higher sensitivity of SW480 cells to ALA-PDT
is at least partially due to the significantly better conversion of
ALA to PpIX by the SW80 cells.[76] The stronger
phototoxicity observed here at the same ALA dose may be due to the
compositional difference of the carrier QD.Cationic AIS-PEI/2MPA
QDs and their ALA-loaded versions were tested
between 0.007 and 0.015 mM ALA doses (0.6–2.24 μg/mL
[cation]) due to the QD-based dark toxicity at higher concentrations
(Figure S12). At these concentrations,
ALA or the cationic AIS QDs showed no dark toxicity in either cell
line (Figure e,g).
Significant dark toxicity was only recorded at 0.015 mM ALA in the
SW480 cell line. Irradiation of the AIS-PEI/2MPA-1-treated cells did
not cause a significant change in the viability with respect to the
dark toxicity of these cationic QDs. At these concentrations, ALA
did not cause notable phototoxicity either. However, phototoxicity
of ALA delivered by the AIS-PEI/2MPA-50%ALA QDs effectively reduced
the viability even at the 0.007 mM ALA dose to 57 and 58% in the HT29
and SW480 cell lines, respectively (Figure f,h). At 0.015 mM ALA concentration, the
viability of the HT29 cells were 60 and 40% when treated with the
AIS-PEI/2MPA-1-30%ALA and AIS-PEI/2MPA-1-50%ALA QDs, respectively.
The SW480 cell line showed a similar trend with ∼65 and 45%
viability after treatment with the AIS-PEI/2MPA-1-30%ALA and AIS-PEI/2MPA-1-50%ALA
QDs. The viability of ALA loaded to the cationic PEG–chitosan
nanoparticles in the study of Chung et al. reduced the viability of
the CT26 cells to 40% at 0.1 mM [ALA] (1.8 J/cm2) while
we reached the same viability after PDT at 0.015 mM [ALA] AIS-PEI/2MPA-1-50%ALA
QDs.[46]All of the further in vitro
experiments were performed at 0.35
mM ALA and corresponding concentrations of the AIS-2MPA-3 QDs as well
as at 0.015 mM ALA and the corresponding amounts of the AIS-PEI/2MPA-1
QDs because at these doses, the 2D experiments indicated no dark toxicity
but significant phototoxicity on both cell lines (Figure i–l).PDT was
also tested on the 3D spheroid constructs of the HT29 and
SW480 cells treated with ALA, AIS QDs, and their ALA-loaded formulations.
Free ALA (0.015 and 0.35 mM) reduced the viability to ∼70–75%
in both the HT29 and SW480 cells after irradiation. Both QDs improved
the ALA-based PDT: The viability of the cells treated with the AIS-2MPA-3-50%ALA
QDs (0.35 mM ALA) reduced the viability of the HT29 cells to 45% and
SW480 cells to 40% (Figure i,j). In the cationic AIS-PEI/2MPA-3-50%ALA QDs, irradiation
of the treated spheroids reduced the viability of the HT29 and SW480
cells to 55 and 45%, respectively, at 0.015 mM ALA concentration (Figure k,l).Because
irradiation of free ALA and free QDs did not create significant
phototoxicity and the ALA-loaded ones showed dose-dependent toxicity,
ROS generation due to irradiation of the intracellular PpIX should
be the primary factor responsible for the reduction of cell viability.
To determine the amount of ROS generated after blue light illumination,
a cell-permeable nonfluorescent dye DCFDA is utilized as the ROS indicator.
The ROS oxidizes the dye to green fluorescent dichlorofluorescein
(DCF). After incubation of the HT29 and SW480 cells with ALA, QDs,
and ALA-loaded QDs, the production of ROS was followed by the green
fluorescence intensity at 538 nm (Figure S17a,b). QD irradiation did not generate any ROS, which supports no phototoxicity
observation in the absence of ALA. The ALA-loaded QDs showed significantly
more ROS generation than free ALA in both cell lines, especially with
50% ALA loading to QDs. The amounts of the ROS generated by ALA-loaded
cationic versus ALA-loaded anionic QDs are not significantly different,
although the anionic ones carried more ALA at the studied doses of
the two QDs (0.0.015 versus 0.35 mM ALA). The release of ALA from
the cationic QDs after 24 h was only about 10% more than the ALA released
from the anionic QDs (Figure S11c,d). At
especially low ALA concentrations, the amount of PpIX produced from
0.015 and 0.35 mM ALA is similar (Figure S15). These two data support a similar amount of ROS generated by ALA
delivered by either delivery vehicle upon irradiation. More toxicity
via the cationic delivery vehicle was observed when the phototoxicity
of the ALA-loaded QDs is at similar ALA concentrations, but the cationic
versus anionic QD delivery was considered. For example, at 0.07 mM
ALA delivered by cationic AIS-PEI/2MPA-1-50%ALA versus anionic AIS-2MPA-3-50%ALA,
the viabilities of both cells were around 15–30% versus 20–30%,
respectively. Considering no dark toxicity of the anionic QD but significant
dose-dependent cytotoxicity of the cationic QD, the anionic AIS-2MPA
QDs are better delivery vehicles when the above discussion is also
taken into account.To further confirm the therapeutic efficiency
of the nanoparticles
and PDT-dependent cell death, a calcein-AM/propidium iodide (PI) staining
was used. No dead cells were seen in the absence of laser treatment
at the studied doses of QDs and ALA. Treatment with the cationic or
anionic AIS QDs followed by irradiation did not cause any cell death
either. Few dead cells were observed when treated with the ALA-loaded
cationic AIS QDs only in the SW480 cell line but not with the ALA-loaded
anionic AIS QDs. However, the ALA-loaded cationic and anionic AIS
QDs exhibit significantly higher cell death after irradiation both
in the 2D cell cultures and 3D spheroid constructs of both cell lines. Figure a,b clearly shows
more cell death when the AIS-2MPA-3-50%ALA QDs were used, consistent
with the cell viability results and measured ROS levels.
Figure 6
Live/dead images
of HT29 and SW480 (a) 2D and (b) 3D-spheroid cultures.
The cultures were treated with free ALA (0.35 mM), AIS-2MPA-3, AIS-2MPA-3-30%ALA,
and AIS-2MPA-3-50%ALA QDs at 50 μg/mL and free ALA (0.015 mM),
AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and AIS-PEI/2MPA-1-50%ALA at
2 μg/mL after 24 h incubation with/without PDT illuminated at
420 nm with a blue lamp for 5 min. Apoptotic and necrotic-induced
cell death in (c) the 2D and (d) 3D cultures of the SW480 cells. Comparison
of the cell death pathways induced after PDT (420 nm with a blue lamp
for 5 min) with free ALA (0.35 mM), AIS-2MPA-3, AIS-2MPA-3-30%ALA,
and AIS-2MPA-3-50%ALA QDs at 50 μg/mL and free ALA (0.015 mM),
AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and AIS-PEI/2MPA-1-50%ALA at
2 μg/mL. Annexin-V was used to indicate apoptosis (green), and
propidium iodide was used to indicate necrosis (red). “Control”
indicates the untreated cells. Scale bars for the images are 400 μm.
Live/dead images
of HT29 and SW480 (a) 2D and (b) 3D-spheroid cultures.
The cultures were treated with free ALA (0.35 mM), AIS-2MPA-3, AIS-2MPA-3-30%ALA,
and AIS-2MPA-3-50%ALA QDs at 50 μg/mL and free ALA (0.015 mM),
AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and AIS-PEI/2MPA-1-50%ALA at
2 μg/mL after 24 h incubation with/without PDT illuminated at
420 nm with a blue lamp for 5 min. Apoptotic and necrotic-induced
cell death in (c) the 2D and (d) 3D cultures of the SW480 cells. Comparison
of the cell death pathways induced after PDT (420 nm with a blue lamp
for 5 min) with free ALA (0.35 mM), AIS-2MPA-3, AIS-2MPA-3-30%ALA,
and AIS-2MPA-3-50%ALA QDs at 50 μg/mL and free ALA (0.015 mM),
AIS-PEI/2MPA-1, AIS-PEI/2MPA-1-30%ALA, and AIS-PEI/2MPA-1-50%ALA at
2 μg/mL. Annexin-V was used to indicate apoptosis (green), and
propidium iodide was used to indicate necrosis (red). “Control”
indicates the untreated cells. Scale bars for the images are 400 μm.Apoptotic/necrotic cell death caused by the PDT
treatment of the
cells was also determined. The SW480 cells in the 2D and 3D models
were stained with Annexin-V to detect apoptosis (shown in green) and
PI for detection of necrosis (shown in red) 24 h after illumination.
ALA showed apoptotic cell death in 2D and a combination of apoptotic
and necrotic cell death in 3D. Dramatic enhancement in the apoptotic
cell population was observed with the ALA-loaded AIS QDs both in the
2D and 3D cell cultures (Figure c,d). QDs with 50% ALA loading caused a higher population
of necrotic/apoptotic cells than the 30% ALA-loaded ones. Necrotic/apoptotic
cells were more visible in the 3D spheroid and more with the cationic
nanoparticles (Figure d).
Conclusions
A portfolio of the emission tunable, cationic,
and anionic AIS
QDs was successfully prepared using a one-step, RT, aqueous synthesis
method using 2MPA or PEI/2MPA as the coating/stabilizing agents for
the first time in the literature. The best precursor stoichiometry
for the synthesis of both the anionic and cationic AIS QDs with small
sizes (less than 8 nm) and the strongest emission at 630–617
nm with QYs 19.4% (AIS-2MPA-3) and 20.3% (AIS-PEI/2MPA-1) was determined
as Ag/In/S 1/10/10 at a coating/cation ratio of 5 in the cation-rich
formulations. To the best of our knowledge, these are among the highest
reported QYs for AIS, which lacks the Zn dopant or ZnS shell. Moreover,
these QDs showed excellent colloidal stability with enhanced emission
intensity over time. Although emission tunability was observed, strong
emission around 700 nm was not achieved. This may be studied further
by changing the coating/cation ratio and/or PEI/2MPA ratio in the
future.The in vitro studies showed that both the AIS QDs are
internalized
by various cancer cells (HeLa, HCT116, SW490, and HT29) and exhibit
strong intracellular luminescence above 600 nm (within the optical
imaging window) upon 488 nm excitation, proving their efficiency in
medical imaging. The cationic AIS QDs were internalized slightly more
than the anionic ones by all cell types but were also more toxic.
Because the AIS-2MPA QDs caused no significant cytotoxicity up to
100 μg/mL [cation], the AIS-PEI/2MPA QDs reduced the viability
of the cells above 2 μg/mL [cation].After electrostatic
loading of ALA to the QDs at two different
concentrations (30 and 50% ALA with respect to the coating amounts),
both QDs released ALA preferentially in acidic pH (up to 80% after
30 h) with less than 10% release at the physiological pH. Hence, the
acidic tumor microenvironment could enhance the ALA release at the
tumors selectively, thereby enhancing tumor localization and subsequently
enhancing the conversion of ALA to PpIX.A dose-dependent phototoxicity
surpassing the phototoxicity of
free ALA was observed after PDT with a 420 nm blue lamp for 5 min
in either cationic or anionic AIS QDs. Reduction in cell viability
was correlated with ROS generation and apoptotic/necrotic cell death.
In the 3D spheroids, while 0.35 mM free ALA reduced the viability
by about 25–30% in both cells lines, the anionic AIS QDs with
50% ALA loading reduced it by about 55–60%. Similarly, 0.015
mM ALA delivered by the cationic QDs loaded with 50% ALA caused 45–55%
reduction of the cell viability. In the 2D cell cultures, phototoxicity
was even greater, reacting to 70–80% reduction in viability.
Thus, the IC50 values of the ALA were reduced significantly when delivered
with the AIS QDs.In terms of comparing the cationic and anionic
AIS as a delivery
vehicle for ALA, the data suggest that they are comparable; however,
intrinsically higher toxicity of the cationic one (due to the presence
of PEI) requires lower doses, which may be even advantageous if, for
example, coupled with molecular targeting of the tumors in the future.
Alternatively, anionic AIS appear to offer a safe delivery vehicle.In the clinical scenario, the tumor selectivity of such multimodal
theranostic nanoparticles will also be aided by the EPR effect, which
promotes the accumulation of the nanoparticles and hence ALA at the
tumor site. This would lead to the enhanced release and conversion
of ALA to PpIX in the tumor cells owing to the faster release of ALA
at the acidic tumor microenvironment coupled with higher conversion
of ALA to PpIX in the tumor cells, thereby inducing higher phototoxicity
to the tumor cells when irradiated. In addition, another level of
tumor selectivity may be achieved by tagging these QDs with tumor-specific
ligands, such as folic acid, anti-Her2, or anti-EGFR antibodies.[3,77,78]Furthermore, considering
the benefits observed in combination therapies,
the AIS QDs loaded with ALA and an antibiotic or anti-cancer drug
may dramatically enhance the treatment of such difficult to treat
diseases.[77] These cationic and anionic
AIS QDs loaded with ALA or other PDT agents also have significant
potential in antibacterial/antiviral PDT.Hence, these cationic
and anionic AIS QDs with strong and stable
luminescence above 600 nm with strong intracellular optical signals
to provide image-guided therapy and capacity to deliver the therapeutic
agents emerge as easy to make promising theranostic nanoparticles.
Authors: Grzegorz Gabka; Piotr Bujak; Kamila Giedyk; Andrzej Ostrowski; Karolina Malinowska; Jerzy Herbich; Barbara Golec; Ireneusz Wielgus; Adam Pron Journal: Inorg Chem Date: 2014-05-01 Impact factor: 5.165
Authors: Hans C Arora; Mark P Jensen; Ye Yuan; Aiguo Wu; Stefan Vogt; Tatjana Paunesku; Gayle E Woloschak Journal: Cancer Res Date: 2011-12-12 Impact factor: 12.701
Authors: Ajmeeta Sangtani; Eleonora Petryayeva; Miao Wu; Kimihiro Susumu; Eunkeu Oh; Alan L Huston; Guillermo Lasarte-Aragones; Igor L Medintz; W Russ Algar; James B Delehanty Journal: Bioconjug Chem Date: 2017-12-21 Impact factor: 4.774
Scheme 1
Figure 1
Figure 2
Figure 3
Figure 4
Figure 5
Figure 6