Feng Zhang1,2, Zhiyu Liu2, Xijing He1, Zhanqi Li2, Bin Shi2, Fengmei Cai3. 1. Department of Orthopedics, The Second Affiliated Hospital of Xi'an Jiaotong University, Xi'an, China. 2. Department of Orthopedics, Xi'an Fourth Hospital, Xi'an, China. 3. Department of Pathology, Xi'an Fourth Hospital, Xi'an, China.
Abstract
Rheumatoid arthritis (RA), autoimmune disease that is categorized via chronic inflammation manifestation, obesity, cardiovascular risk and even enhanced the mortality and affect the 0.3 and 1% of population worldwide. The current experimental study was scrutinize the anti-arthritic effect of β-sitosterol loaded solid lipid nanoparticles (SLN) against complete Fruend adjuvant (CFA)-induced arthritis via dual pathway. Double emulsion solvent displacement method was used for the preparation of β-sitosterol solid lipid nanoparticles (SLN). CFA was used to induce arthritis and rats were divided into different groups for 28 days. Biochemical, anti-inflammatory, pro-inflammatory cytokines and inflammatory mediator were estimated, respectively. Receptor activator of nuclear factor kappa-B ligand (RANKL), signal transducer and activator of transcription-3 (STAT3) nuclear factor erythroid 2-related factor 2 (Nrf2), Heme Oxygenase-1(HO-1) and Nuclear factor-κB (NF-κB) expression were estimated. β-sitosterol-SLN significantly (p < .001) reduced the paw edema, arthritic index and increased the body weight. β-sitosterol-SLN increased the redox status of synovium {reduce the malonaldehyde (MDA) and increase superoxide dismutase (SOD), glutathione (GSH) and catalase (CAT)} level and reduced the cytokines such as tumor necrosis factor-α (TNF-α), interleukin-1β (IL-1β), interleukin-2, interleukin-6, interleukin-16, interleukin-17 and increased level of interleukin-10, Transforming growth factor beta (TGF-β). β-sitosterol-SLN significantly (p < .001) reduced the level of cyclooxygenase-2 (COX-2), prostaglandin E2 (PGE2), vascular Endothelial Growth Factor (VEGF) and NF-κB. β-sitosterol-SLN significantly increased the expression of HO-1,Nrf2 and decreased the expression of NF-κB, RANKL, STAT3. In conclusion, β-sitosterol SLN showed the antiarthritic effect via suppression of NF-kB and activation of HO-1/Nrf-2 pathway.
Rheumatoid arthritis (RA), autoimmune disease that is categorized via chronic inflammation manifestation, obesity, cardiovascular risk and even enhanced the mortality and affect the 0.3 and 1% of population worldwide. The current experimental study was scrutinize the anti-arthritic effect of β-sitosterol loaded solid lipid nanoparticles (SLN) against complete Fruend adjuvant (CFA)-induced arthritis via dual pathway. Double emulsion solvent displacement method was used for the preparation of β-sitosterol solid lipid nanoparticles (SLN). CFA was used to induce arthritis and rats were divided into different groups for 28 days. Biochemical, anti-inflammatory, pro-inflammatory cytokines and inflammatory mediator were estimated, respectively. Receptor activator of nuclear factor kappa-B ligand (RANKL), signal transducer and activator of transcription-3 (STAT3) nuclear factor erythroid 2-related factor 2 (Nrf2), Heme Oxygenase-1(HO-1) and Nuclear factor-κB (NF-κB) expression were estimated. β-sitosterol-SLN significantly (p < .001) reduced the paw edema, arthritic index and increased the body weight. β-sitosterol-SLN increased the redox status of synovium {reduce the malonaldehyde (MDA) and increase superoxide dismutase (SOD), glutathione (GSH) and catalase (CAT)} level and reduced the cytokines such as tumor necrosis factor-α (TNF-α), interleukin-1β (IL-1β), interleukin-2, interleukin-6, interleukin-16, interleukin-17 and increased level of interleukin-10, Transforming growth factor beta (TGF-β). β-sitosterol-SLN significantly (p < .001) reduced the level of cyclooxygenase-2 (COX-2), prostaglandin E2 (PGE2), vascular Endothelial Growth Factor (VEGF) and NF-κB. β-sitosterol-SLN significantly increased the expression of HO-1,Nrf2 and decreased the expression of NF-κB, RANKL, STAT3. In conclusion, β-sitosterolSLN showed the antiarthritic effect via suppression of NF-kB and activation of HO-1/Nrf-2 pathway.
Rheumatoid arthritis (RA), autoimmune disease that is categorized via chronic inflammation
manifestation, obesity, cardiovascular risk and even enhanced the mortality and affect the
0.3 and 1% of population worldwide. RA categorized via inflammation, synovial membrane,
swelling cartilage destruction, autoantibody production and bone destruction. Research
suggest that the RA mostly affect the middle-aged females (50–60 years) and women are most
affected as compared to man (Rutherford et al., 2017). RA is also liked with the systemic complications, early mortality,
socioeconomic cost and disability. During the expansion of RA, its affects the hands joints
and feet resultant in a steady painful swelling, pannus formation, abnormal expansion of
synovium, exaggerate and changes in the joint morphology (Funk et al., 2006). The exact initiation mechanism of arthritis is still not fully
clear, but some researcher and previous publish report suggest that the various
pro-inflammatory cytokines, immune cell populations and inflammatory mediators is admitted.
During the pathological process and early symptoms of swelling, heat, reduced joint function
and pain; the later stage exhibit different degrees of deformity and joint stiffness
accompanying bone damage and disability risk (Woodruff et al., 2002; Funk et al., 2006;
Petchi et al., 2015). Research suggests that
inflammation is a physiological reaction against harmful stimuli, such as pathogens in the
body. By inducing the release of signaling molecules, inflammation has a protective effect
that deactivates various deleterious pathogens (Funk et al., 2006; Amresh et al., 2007;
Jalalpure et al., 2011).Currently, no effective treatment is available for the RA, but the clinical and physician
used the non-steroidal anti-inflammatory drugs (NSAIDs), disease modifying and
glucocorticoids drug for the treatment (Kumar et al., 2015a,b). Conversely, recent advancement, NSAIDS is the choice of drug but these
therapies having the limitation due to their side and adverse effects like cardiac toxicity
and gastrointestinal effects. Another treatment glucocorticoid showed the side effects like
metabolic disorder and osteoporosis. In the recent year, the researcher targeted the
pro-inflammatory cytokines and inflammatory mediators to treat the RA and its complication.
Previous research suggest that the macrophage play a defence role against the invading agent
such as viruses, fungi and bacteria (Kumar et al., 2015a,b, 2016b). Due to the invading
agent attack, start the secretion of cellular signaling molecules and numerous
pro-inflammatory cytokines such as tumor necrosis factor-α (TNF-α), interferon-γ (IFN-γ),
interleukin-6 (IL-6) and interleukin 1-β (IL-1β) and inflammatory mediators like
prostaglandin E2 (PGE2), nitric oxide (NO) and cyclooxygenase-2 (COX-2). Moreover,
de-regulated cytokine production and induction of inflammation are liked with the conditions
viz., diabetes, arthritis, cancer, obesity and cardiovascular disease. Therefore, urgent
need of one effective therapeutic agent to treat the arthritis via regulation the production
of pro-inflammatory mediators (Kumar et al., 2016a; Rahman et al., 2016, 2017). Published literature suggests that numerous
inflammatory cells are present to infiltrate the affected RA inflammatory sites of patients
suffering from pro-inflammatory cytokines, such as IL-6, which catalyzes the spread of
native CD4+ cells to the T helper of 17 lymphocytes by enhancing signal transducer and
transcription activator-3 (STAT-3) and intracellular expression (Sengupta et al., 2011; Kamel et al., 2018).Pro-inflammatory cytokines, such as IL-17, play a crucial role in the expansion and decline
of RA via boosting the synovial fibroblasts and immune cells along with boosting the
expression of nuclear factor (NF-κB) and down-regulating the cascade such as inflammatory
mediators like TNF-α (Sengupta et al., 2011;
Kamel et al., 2018). IL-17 increases the
production of reactive oxygen species (ROS). Significantly, pro-inflammatory cytokines like
TNF-α, ROS, and IL-17 are functioning synergistically, inducing expression of vascular
endothelial growth factor (VEGF). Previous research has reported that VEGF plays a crucial
role in the inflammatory response, and that angiogenesis is also the cause of chronic
rheumatoid inflammation (Sengupta et al., 2011;
Gao et al., 2016; Kamel et al., 2018).Activity induces synoviocytes to induce elevated levels of toxic cytokines such as kappa-B
ligand nuclear factor (RANKL) and matrixmetalloproteinase-3 (MMP-3). RANKL is a crucial
enzyme for RA cartilage pathology destruction, as proteoglycs and the form of collagens (IX
and X) are digested. MMP-3 is the principal cause of bone degradation in RA and functions as
a differentiating osteoclastic cause (Arham et al., 2016; Kamel et al., 2018).As in the case of various natural compounds, poor aqueous solubility, resulting in low
bioavailability and low targeting efficacy, has restricted clinical development of
production of β-Sitosterol. Its well documented that nanoparticle drug delivery system
increases the therapeutic efficacy of various natural compounds. Several new
nano-formulations have been used in a recent study to improve the therapeutic potential of a
large number of naturally derived drugs such as umbelliferone, resveratrol, vincristine,
curcumin, silymarin rutin, paclitaxel, artemisinin, camptothecin, honokoil and green tea
catechins (Bilia et al., 2017). Many of these
natural products are already on the market, others are undergoing clinical trials (Bilia
et al., 2017).As my knowledge, few of the studies have been carried out on the β-sitosterol to improve
the therapeutic efficacy. Most of the investigations conducted with β-sitosterol have
focused on using it and its derivatives as an excipients to regulate drug release or promote
drug absorption (Farkas et al., 2006; Lacatusu
et al., 2012). In previous study, cyclodextrins
has been used to increase the aqueous bioavailability and solubility of β-sitosterol.
Imanaka et al., showed that the liposomal containing formulation of β-sitosterol enhanced
the natural killer cell activity and reduced the B16BL6melanoma cells colonies in the lungs
of experimental mice (Imanaka et al., 2008). Awad
et al., showed the protective effect of β-sitosterol against various cancer cells via
involving the 2-hydroxypropyl-β-cyclodextrin (HP-βCD) as a carrier vehicle (Awad et al.,
2000, 2001, 2007). These investigations
showed that β-sitosterol reduced the cell proliferation after the 3–5 days at 16–32 µM. It
is well documented that cyclodestrins commonly used in the pharmaceutical preparations as
excipients to increase the bioavailability and solubility. We hypothesized that solid lipid
nano-particles of β-sitosterol can offer better enhancement of antiarthritic effect against
the rodent model. This assumption is due to various beneficial effect of SLN such as
improved drug-loading capacity, controlled release, facilitated, improved solubility and
targeted drug release.Solid lipid nanoparticles (SLNs) are the most promising oral drug delivery carriers due to
their long term stability, high drug-loading capacity, excellent biocompatibility,
large-scale production viability and long-term stability. Furthermore, previous researcher
suggests that the SLN increased the intracellular drug delivery for anti-arthritic drugs
(Arora et al., 2015; Ahmad et al., 2018). SLNs are a colloidal system primarily
formulated of solid lipids. SLNs get the more popularity against the numerous poorly soluble
drugs such as anti-arthritic drug.With regard to research work carried out in literature to boost β-sitosterol
biopharmaceutical efficiency using nanocarriers, the specific formulation such as
PLGA-loaded β-sitosterol nanoparticles (Andima et al., 2018). While these discuss formulation exhibited a definite improvement in the
drug's biopharmaceutical attributes, the current investigation was undertaken to discuss the
significant finding of β-sitosterol-SLNs systematically optimized to enhance the
effectiveness of drug therapy against CFA-induced arthritis.
Material and methods
Chemical
Complete Fruend’s adjuvant (CFA) was procured from the Chondrex, Inc. (U.S.).
Lipopolysaccharides (LPS), indomethacin and β-sitosterol were purchased from the Sigma
Chemical Company, St. Louris, MO, U.S.A. IL-1β, IL-6, IL-10, IL-16, IL-17 and TNF-α were
purchased from the U-CyTech Biosciences. Rest of the chemical used in the current
experimental study were procured from the reputed vendors.
Preparation of the β-sitosterol-Solid lipid nano-particle of
(β-sitosterol-SLNs)
Solvent diffusion and hot homogenization model was used for the fabrication of SLN of
β-sitosterol via using the previous reported protocol with some modification. The quantity
of solid lipid was used for the formulation of SLN was selected on the solubility basis.
250 mg Compritol 888 ATO, 60 mg Phospholipid 90 G (PL90G) was used for the formulation of
solid lipid. Both the co-surfactant and solid lipid were melted upto 70 °C and fixed
amount of β-sitosterol (50 mg) were added with continuous stirring for complete soluble in
the liquid (lipidic). After that, tween 80 (3% w/v) solutions was separately prepared
(soluble in the 10 mL). The aqueous phase was dissolved into the organic phase under the
continuous homogenization for 2–6 min at 10000 rpm to obtain the uniform dispersion.
Additionally, 10 mL of water added into the solvents and then constantly stirred for 1–4 h
at 1600 rpm in ice bath for acquisition of SLNs and finally SLNs kept in the refrigerator
for further use.
Characterization of β-sitosterol-Solid lipid nano-particle of
(β-sitosterol-SLNs)
Particle size (PS)
Dynamic light dispersion technique (M/s Malvern Instruments, Worcestershire, UK) was
used for the determination of particle size distribution of β-sitosterol-SLNs.
Drug loading capacity (LC) and entrapment efficiency (EE)
The loading capacity and entrapment efficiency are well known proportion of drug
effectively struck in the SLNs. The LC and EE were estimated via using the previous
reported method of Rahman et al., with minor modification (Rahman et al., 2019). In brief, 2 mL dispersion aliquot of SLN
was ultra-centrifuged and supernatant discarded and collected the pallet. Additionally,
pellet comprising SLN was finally applied for ultrasonication for 15 min to complete
remove the drug from formulation. Finally, the drug collected in mobile phase and
estimated via high-performance liquid chromatography (HPLC). The below given equation
was used for the estimation of loading capacity and entrapment efficiency.
Transmission electron microscopy (TEM)
The 1 mL aliquot of SLNs was 100 time diluted with the triple distilled water and
finally distributed on the copper grid with phosphotungstic acid solution (1%), and
finally, the prepared sample was observed under the transmission electron microscope
(JEM-2100F, M/s Jeol, Tokyo, Japan).
In vitro drug release study
In vitro drug release study was carried out to estimate the
release pattern of β-sitosterol-SLNs. Briefly, the SLNs dissolved in phosphate buffer
saline (PBS; pH-7.4) at 37 °C at 100 rpm for 24 h. finally the SLN was packed in the
dialysis bag. 2.5 mg of SLN dispersion was loaded into the dialysis bag and used for the
current experimental study. 0.5 mL aliquot of the samples were taken at regular time
interval and finally loaded the equal amount of fresh medium at 37 °C. HPLC spectroscopy
was used for analyzed the sample and estimation the percent drug release. The received
drug release was fitted with different mathematical model includes zero, first, Higuchi
and Korsmeyer – Peppas model to scrutinize the release kinetic pattern.
Stability studies
The stability study was carried out at 25 °C/60% RH and 40 °C/75%RH for estimation the
stability of formulation. Briefly, the formulation was kept in the tight-sealed vials and
subjected to perform the stability studies at different time interval (0, 1, 2, 4, 8 and
12 weeks). These formulations are scrutinized for different parameter such as PDI, PS, LC
and EE at different time intervals.
Experimental rodent
Swiss Wistar rats (150–190 g, sex – male) used for the current experimental study. All
the experimental study was carried out according to the Institutional guidelines. All the
experimental rats kept in the standard laboratory condition such as 22 ± 5 °C temperature;
60–75% relative humidity and 12-h dark and light cycle.
Induction of arthritis via complete freund’s adjuvant (CFA)
Complete Freund’s adjuvant (CFA) was used for the induction of arthritis. 0.1 ml
injections of Wistar rats were injecting the CFA in the right hind metatarsal foot pad
with equal volume of saline in the rat control group. The day of injection, day 0
immunization.
Drug administration
Tested and standard drug were suspended into the 1% solution of carboxyl methyl cellulose
(CMC) and orally administered to the experimental rats for 28 days. Normal control group
rats received the 1% solution of CMC.
Experimental protocol
The experimental rats were divided into different groups as followsGroup I: Normal controlGroup II: CFA received onlyGroup III: CFA + β-sitosterol (2.5 mg/kg)Group IV: CFA + β-sitosterol (25 mg/kg)Group V: CFA + β-sitosterol-SLNGroup VI: CFA + Indomethacin (400µg/kg)The rats were received the over mention treatment for 28 days. The paw edema, body
weight, water and food intake were estimated at regular time intervals. At end of the
experimental study, the rats were anesthetized and blood samples were withdrawn via
puncturing the retro orbital (Kumar et al., 2015a,c).
Index of spleen and thymus
At end of the experimental study period, the rats were scarified via using the excess of
anesthesia and immediately thymus and spleen tissue was successfully removed from the all
group of animals and weighted. For the estimation of thymus and spleen index, the index
was presented at a ratio (mg/g) weight versus body weight, respectively.
Poly-arthritic index
The arthritis index and paw swelling were screened regularly in order to determine the
extent of arthritis. Plethysmometer was used for the estimation of paw swelling and the
data was presented in the form of paw volume calculated via subtracting the basal volume.
Previously used method was used for the estimation of inflammation in the paw via given
the score. Score 0: paws have no swelling or may be focal redness; score 1: figure joint
persist the swelling; score 2: swelling of the wrist joints or ankle; score 3: expand
inflammation of entire paw and score 4: paws ankylosis or deformity. Each paw was
calculated separately and the cumulative scores of 4 paws of each rat were used as
polyarthritis index with a maximum value of 16 per rat.(Kumar et al., 2015a,c, 2016b).
Antioxidant parameters
For the biochemical parameter estimation, the tissue was successfully removed from
excised ankle joint all experimental group rats weighted and stored at −80 °C. Further,
the tissue homogenate (10%) was prepared in phosphate buffer saline and used for the
estimation of catalase (CAT), malonaldiadehyde (MDA), superoxide dismutase (SOD) and
glutathione (GSH), respectively.
Hematological parameters
Hematological parameters such as erythrocyte sedimentation rate (ESR), white blood cells
(WBC), hemoglobin (Hb) and red blood cells (RBC) were estimated using the previous
reported method with minor modification (Jalalpure et al., 2011; Kumar et al., 2016b).
Hepatic parameters
Hepatic parameters such as Aspartate transaminase (AST), alkaline phosphatase (ALP) and
Alanine transaminase (ALT) were estimated using the colometric kits (JOURILABS kit).
Cytokines estimation
ELISA kits were used for estimating pro-inflammatory cytokines including IL-6, IL-1β,
IL-10, Il-16, IL-17 and TNF-α (U-CyTech Biosciences) were estimated following the
manufacture instruction. Pro-inflammatory cytokines were estimated in the serum were
estimated pg/ml and in tissue was estimated pg/mg.
Inflammatory mediators
Inflammatory mediators such as NF-κB, COX-2, VEGF and PGE2 were estimated
using the ELISA kits following the manufacture instruction.
Quantitative RT-PCR
SV total RNA isolation system was used for separation of total RNA from the high limb
tissue of rats (Promega, Madison, WI, USA). The purity of RNA was confirmed via using the
spectrophotometer at 260 nm. RT-PCR kit was used for reverse transcribed into cDNA
(Stratagene, Santa Clara, CA) using the manufacture instruction. Briefly, QuantiFast SYBR
Green PCR master mix (25 μl) mix with primer pair mix (2 μl), dH2O (22.5 μl)
and cDNA (0.5 μl) and maintain the final volume 50 μl. The sequences of the primer listed
in Table 1. PCR included 95 °C for 10 min
activate the AmpliTaq DNA polymerase, followed via 40 cycles for 15 s at 95 °C
(denaturing) and 1 min at 60 °C (extension/annealing). The results were presented in cycle
threshold (Ct), where the enhanced fluorescence curve passes across a threshold
value.
Table 1.
The list of primer.
S. No
Gene/
Primer
Reverse
Forwarded
1
HO-1
CCTCTGGCGAAGAAACTCTGTC
ACCCCACCAAGTTCAAACAGC
2
Nrf-2
TCGGCTGGGACTTGTGTTCAGT
GCCTTCCTCTGCTGCCATTAGT
3
NF-kB
GAGGAAGGCTGTGAACATGAGG
TTCTGGTGCATTCTGACCTTGC
4
RANKL
GAAGGGTTGGACACCTGAATGC
CACACCTCACCATCAATGCTGC
5
STAT-3
TGACCTGCCACCTGACAGTA
GTAGGGGTTCCTCACCCTTC
6
GAPDH
AGACAGCCGCATCTTCTTGT
TGGAAGATGGTGATGGGTTT
The list of primer.
Statistical analysis
All the data provided in the current experimental analysis as means ± Standard Medium
Error (SEM). One-way analysis of variance (ANOVA) was used for comparison between the
various groups, followed by comparison testing with Dennett. When p < .05 was perceived to be substantial difference. GraphPad Prism software
was used for the statistical analysis.
Result
Validation of optimized model
The prepared β-sitosterol-SLN nanoparticles were found in the spherical shape with
uniform in size distribution. The formulated nano-particles optimized via using the
various parameters like particle size in size, showing the validly of predicted model. The
prepared β-sitosterol-SLN showed the averaged mean percentage, mean loading capacity and
entrapment efficiency. Transmission electron microscopy (TEN) exhibited the nano size
range and spherical shape of prepared β-sitosterol-SLN (Supplementary figure
1).
In vitro release of β-sitosterol -SLN
In vitro permeation experiment was carried out to
estimation the permeation of β-sitosterol-SLN and control. invitro permeation profile via
excised abdominal rat skin. The β-sitosterol-SLN skin permeation profiles complied with
the Fick 's diffusion rule. Statistical analysis for 24 h experimental study, demonstrated
the higher flux for β-sitosterol-SLN as compared to control (β-sitosterol control) (Table 2). Whereas the cumulative amount of
β-sitosterol permeate from SLN was almost 4 times higher as comparison to control.
Table 2.
In vitro skin permeation studies of β-sitosterol-SLN
and control.
Formulation Code
Flux (µg/cm2/
hr)
Permeability Co-efficient ×
10−3(cm/hr)
Enhancement ratio
β-sitosterol -SLN
14.34
1.98
3.98
Control
3.21
0.29
1
In vitro skin permeation studies of β-sitosterol-SLN
and control.
Characterization of β-sitosterol-SLN
The β-sitosterol-SLN exhibited the high LC (14.1%) and EE (90%) presented in the
Supplementary Table
1.
Particle size distribution and polydispersity index (PDI)
The optimized β-sitosterol-SLN particle size stored at 25 °C/60% RH (73.06 to 67) and
40 °C/75% RH (66.01 to 105 nm) presented in the Supplementary Tables 1 and
2. During the storage at 25 °C/60% RH, the particle size of the
β-sitosterol was quite unchanged, while at 40 °C/75%RH the particle size of β-sitosterol
was enhanced due to aggregation phenomenon. However, Supplementary Table
1 showed the low and steady values, thereby at 25 °C/60% RH, showing the
stability of PS for next 12 weeks.
Effect of β-sitosterol-SLN on paw edema
Table 3 exhibited the effect of
β-sitosterol-SLN on the experimental rats. CFA-induced rats demonstrated the increased
paw edema at increase the time and reached maximum at day 21 (3.7 ± 0.69 cm).
CFA-induced rats treated with β-sitosterol (2.5 and 25 mg/kg, body weight) exhibited the
reduction in the paw edema at the day 28 (2.2 ± 0.89 and 1.4 ± 0.93 cm).
β-sitosterol-SLN treated group rats exhibited the maximum diminution in the paw edema
(0.43 ± 0.07 cm). A similar result was obtained for the group treated with
indomethacin.
Table 3.
The effect of β-sitosterol on the paw edema of CFA-induced arthritic rats.
S. No
Groups
Increase in
Joint diameter (cm) (days)
Day 7
Day 14
Day 21
Day 28
1
CFA
2.8 ± 0.43
3.1 ± 0.78
3.7 ± 0.69
3.5 ± 0.72
2
CFA+ β-sitosterol
(2.5 mg/kg)
2.1 ± 0.72*
2.5 ± 0.83**
2.4 ± 0.74***
2.2 ± 0.89***
3
CFA+ β-sitosterol
(25 mg/kg)
2 ± 0.84**
2.1 ± 0.45***
1.9 ± 0.45***
1.4 ± 0.93***
4
CFA+ β-sitosterol-SLN
1.4 ± 0.83***
1.2 ± 0.35***
0.82 ± 0.09***
0.43 ± 0.07***
5
CFA + Indomethacin
(400µg/kg)
1.5 ± 0.34***
1.6 ± 0.34***
1.1 ± 0.63***
0.8 ± 0.05***
All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
The effect of β-sitosterol on the paw edema of CFA-induced arthritic rats.All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
Effect of β-sitosterol-SLN on clinical score
Figure 1 exhibited the clinical score of tested
group rats. Normal group did not show the any sign and symptom of clinical score.
CFA-induced rats demonstrated the increased clinical score, which was significantly
down-regulated via β-sitosterol treatment at dose-dependent manner. Indomethacin
treatment showed the reduction in the clinical score.
Figure 1.
The effect of β-sitosterol-SLNs on spleen and thymus index of CFA induced rats.
a: spleen index and b: thymus index. All the data
presented ± SEM. Statistical analysis was performed via One-way ANOVA followed by
Dennett’s test. Where *p˂.05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
The effect of β-sitosterol-SLNs on spleen and thymus index of CFA induced rats.
a: spleen index and b: thymus index. All the data
presented ± SEM. Statistical analysis was performed via One-way ANOVA followed by
Dennett’s test. Where *p˂.05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
Effect of β-sitosterol-SLN on body weight
Body weight is the major factor to estimate the disease progression. Table 4 demonstrated the impact of normal and
experimental rats on body weight. Normal rats showed the increased body weight from
initial body weight (155.4 ± 3.92 gm) to final body weight (190.6 ± 4.98 gm). CFA
induced rats exhibited the increased body weight on first 7 days (158.3 ± 4.98 gm) and
after that showed the reduced body weight to every next 7 days {day 21 (155.8 ± 5.03 gm)
and day 28 (151.3 ± 3.94 gm)}. j-SLN significantly (P < 0.001) increased the body weight {initial body weight (155.3 ± 3.45 gm)
to final body weight (188.5 ± 4.08 gm)}. A similar result was obtained for the group
treated with indomethacin.
Table 4.
The effect of β-sitosterol on the body weight of CFA induced arthritic rats.
S. No
Groups
Body Weight
(gm)
Day 7
Day 14
Day 21
Day 28
1
NC
152 ± 3.45
164.3 ± 2.98
176.4 ± 4.32
190.6 ± 4.98
2
CFA
155.4 ± 3.92
158.3 ± 4.98
155.8 ± 5.03
151.3 ± 3.94
3
CFA+ β-sitosterol
(2.5 mg/kg)
154.5 ± 3.85ns
159.8 ± 4.11ns
164.5 ± 4.38*
169.5 ± 3.94**
4
CFA+ β-sitosterol
(25 mg/kg)
153.9 ± 2.93ns
160.2 ± 3.07*
167.8 ± 3.94*
175.4 ± 4.32**
5
CFA+ β-sitosterol-SLN
155.3 ± 3.45ns
163.4 ± 3.94*
172.4 ± 4.34**
188.5 ± 4.08***
6
CFA + Indomethacin
(400µg/kg)
154.6 ± 3.73ns
1.63 ± 2.93*
171.3 ± 3.45**
186.8 ± 3.84***
All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
The effect of β-sitosterol on the body weight of CFA induced arthritic rats.All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
Effect of β-sitosterol-SLN on arthritic score
Arthritic score is the important parameter for the estimation of arthritis. The
arthritic score of each group rat was shown in Table
5. Normal group rats showed no signs of arthritic score. CFA-induced group rats
showed the arthritic score and confirm the progression of arthritis. CFA induced showed
the arthritic score 4.1 ± 0.73 (day 7), 5.4 ± 0.89 (day 14), 6.9 ± 0.78 (day 21) and
7.8 ± 0.78 (day 28). β-sitosterol-SLN significantly reduced the arthritic score 3 ± 0.67
(day 7), 2.1 ± 0.54 (day 14), 1.3 ± 0.28 (day 21) and 0.6 ± 0.02 (day 28). A similar
result was observed in the indomethacin group rats.
Table 5.
The effect of β-sitosterol on the arthritic score of CFA-induced arthritic
rats.
S. No
Groups
Arthritic
Score
Day 7
Day 14
Day 21
Day 28
1
CFA
4.1 ± 0.73
5.4 ± 0.89
6.9 ± 0.78
7.8 ± 0.78
2
CFA+ β-sitosterol
(2.5 mg/kg)
3.9 ± 0.78*
4.9 ± 0.78**
5.6 ± 0.83***
4.8 ± 0.78***
3
CFA+ β-sitosterol
(25 mg/kg)
3.5 ± 0.78**
3.4 ± 0.63***
2.9 ± 0.67***
2.5 ± 0.73***
4
CFA+ β-sitosterol-SLN
3 ± 0.67***
2.1 ± 0.54***
1.3 ± 0.28***
0.6 ± 0.02***
5
CFA + Indomethacin
(400µg/kg)
3.2 ± 0.34***
2.3 ± 0.59***
1.7 ± 0.31***
1 ± 0.09***
All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
The effect of β-sitosterol on the arthritic score of CFA-induced arthritic
rats.All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
Effect of β-sitosterol-SLN on spleen and thymus index
During the arthritis, increase the thymus and spleen index is commonly observed.
CFA-induced group exhibited the similar result, showed the increased thymus and spleen
index. β-sitosterol (2.5 and 25 mg/kg) treated group showed the reduction in the thymus
and spleen index. β-sitosterol-SLN demonstrated the maximum reduction of thymus and
spleen index as compared to other treated groups (Figure 1).
Effect of β-sitosterol-SLN on antioxidant parameters
Table 6 showed the effect on the antioxidant
parameters of experimental rats. Normal rats exhibited the TBARS (56.66 ± 2.93 nmol/g),
SOD (5.43 ± 1.02 U/mg protein), CAT (5.34 ± 1.14 U/mg protein) and GSH
(0.39 ± 0.04 µg/g), respectively. CFA induced rats demonstrated the increased level of
TBARS (92.34 ± 4.32 nmol/g) and decreased level of SOD (1.67 ± 0.89 U/mg protein), CAT
(1.76 ± 0.83 U/mg protein) and GSH (0.11 ± 0.02 µg/g). β-sitosterol-SLN significantly
(P < 0.001) reduced the TBARS (59.65 ± 3.43 nmol/g)
and increased the level of SOD (4.75 ± 1.03 U/mg protein), CAT (5.02 ± 0.87 U/mg
protein) and GSH (0.34 ± 0.07 µg/g). A similar momentum was observed in the indomethacin
treated group rats.
Table 6.
The effect of β-sitosterol on the antioxidant parameter of CFA-induced arthritic
rats.
S. No
Groups
Antioxidant
parameters
TBARS (nmol/g)
SOD (U/mgprotein)
CAT (U/mgprotein)
GSH (µg/g)
1
NC
56.66 ± 2.93
5.43 ± 1.02
5.34 ± 1.14
0.39 ± 0.04
2
CFA
92.34 ± 4.32
1.67 ± 0.89
1.76 ± 0.83
0.11 ± 0.02
3
CFA+ β-sitosterol
(2.5 mg/kg)
83.45 ± 2.04*
1.98 ± 0.93*
2.1 ± 0.98*
0.15 ± 0.03*
4
CFA+ β-sitosterol
(25 mg/kg)
72.34 ± 2.93**
2.85 ± 0.99**
3.03 ± 0.94**
0.21 ± 0.04**
5
CFA+ β-sitosterol-SLN
59.65 ± 3.43***
4.75 ± 1.03***
5.02 ± 0.87***
0.34 ± 0.07***
6
CFA + Indomethacin
(400µg/kg)
61.03 ± 2.83***
4.32 ± 1.02***
4.98 ± 0.98***
0.32 ± 0.06***
All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
The effect of β-sitosterol on the antioxidant parameter of CFA-induced arthritic
rats.All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
Effect of β-sitosterol-SLN on hematological parameters
During the arthritic disease, the level of ESR, WBC decrease and the level of Hb, RBC
increase. A similar result was observed in group rats induced by CFA, and
β-sitosterol-SLN altered the hematological parameters close to the normal control (Table 7). A similar result has been observed in
rats of the indomethacin group.
Table 7.
The effect of β-sitosterol on the hematological parameters of CFA-induced arthritic
rats.
S. No
Groups
Hematological parameters
WBC
RBC
Hb
ESR
1
NC
6.45 ± 1.02
8.02 ± 1.04
13.2 ± 1.31
9.04 ± 1.02
2
CFA
8.78 ± 1.12
3.48 ± 1.11
6.75 ± 1.28
14.53 ± 1.04
3
CFA+ β-sitosterol
(2.5 mg/kg)
8.34 ± 1.01*
4.02 ± 1.02**
7.14 ± 0.83*
13.89 ± 0.98**
4
CFA+ β-sitosterol
(25 mg/kg)
7.78 ± 0.98**
6.03 ± 0.85***
8.98 ± 0.91***
12.45 ± 0.78***
5
CFA+ β-sitosterol-SLN
6.76 ± 0.79***
7.84 ± 1.01***
12.8 ± 1.83***
9.34 ± 0.77***
6
CFA + Indomethacin
(400µg/kg)
6.97 ± 0.83***
7.67 ± 0.89***
12.67 ± 1.92***
9.45 ± 0.69***
All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
The effect of β-sitosterol on the hematological parameters of CFA-induced arthritic
rats.All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
Effect of β-sitosterol-SLN on hepatic parameters
Table 8 exhibited the effect of normal and
experimental rats on the hepatic parameters. Hepatic parameters such as AST
(40.3 ± 2.34 U/L), ALT (45.3 ± 1.03 U/L) and ALP (78.5 ± 2.34 U/L) was found in the
normal rats and CFA induced rats showed the increased level of AST (142.3 ± 3.45 U/L),
ALT (170.3 ± 2.12 U/L) and ALP (411.3 ± 6.56 U/L), respectively. β-sitosterol-SLN
significantly (P < 0.001) reduced the level of AST
(50.4 ± 1.89 U/L), ALT (60.3 ± 2.92 U/L) and ALP (100.3 ± 3.84 U/L) and almost similar
result was observed in the indomethacin group rats.
Table 8.
The effect of β-sitosterol on the hepatic parameters of CFA-induced arthritic
rats.
S. No
Groups
Hepatic
parameters
AST (U/L)
ALT (U/L)
ALP (U/L)
1
NC
40.3 ± 2.34
45.3 ± 1.03
78.5 ± 2.34
2
CFA
142.3 ± 3.45
170.3 ± 2.12
411.3 ± 6.56
3
CFA+ β-sitosterol
(2.5 mg/kg)
132.3 ± 4.23*
155.6 ± 3.12**
350.3 ± 4.95**
4
CFA+ β-sitosterol
(25 mg/kg)
100 ± 2.34**
111.3 ± 3.84***
280.4 ± 3.89***
5
CFA+ β-sitosterol-SLN
50.4 ± 1.89***
60.3 ± 2.92***
100.3 ± 3.84***
6
CFA + Indomethacin
(400µg/kg)
55.8 ± 2.93***
69.4 ± 3.01***
111.5 ± 4.56***
All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
The effect of β-sitosterol on the hepatic parameters of CFA-induced arthritic
rats.All values are presented as mean ± SEM. Statisticalanalysis by one-way ANOVA
followed by Dunnett’s multiple comparison. *p < .05, **p < .01 and ***p < .01 vs. Control.
Effect of β-sitosterol-SLN on cytokines
Figure 2 showed the effect of the
β-sitosterol-SLN on cytokine levels of experimental rats serum. CFA induced rats showed
the increased level of TNF-α (170.46 ± 8.46 pg/ml), IL-1β (175.67 ± 6.53 pg/ml), IL-2
(208.04 ± 5.84 pg/ml), IL-6 (156.54 ± 4.34 pg/ml), IL-16 (140.45 ± 5.94 pg/ml), IL-17
(297.45 ± 6.35 pg/ml) and reduced the level of IL-10 (15.43 ± 0.56 pg/ml), TGF-β
(197.45 ± 6.54 pg/ml). β-sitosterol-SLN significantly (p < .001) reduced the TNF-α (60.42 ± 2.35 pg/ml), IL-1β
(50.43 ± 2.04 pg/ml), IL-6 (61.04 ± 2.34 pg/ml), IL-2 (34.05 ± 1.83 pg/ml), IL-16
(30.5 ± 2.38 pg/ml), IL-1β (18.54 ± 3.94 pg/ml), IL-17 (102.5 ± 3.82 pg/ml) and
increased the IL-10 (80.45 ± 2.80 pg/ml), TGF-β (487.94 ± 10.45 pg/ml) as compared to
CFA and other treated group.
Figure 2.
The effect of β-sitosterol-SLNs on cytokines level (Serum) of CFA induced rats.
a: TNF-α, b: Il-6, c: IL-10,
d: IL-2, e: IL-1β, f: IL-16,
g: IL-17 and h: TGF-β. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test.
Where *p˂ .05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
The effect of β-sitosterol-SLNs on cytokines level (Serum) of CFA induced rats.
a: TNF-α, b: Il-6, c: IL-10,
d: IL-2, e: IL-1β, f: IL-16,
g: IL-17 and h: TGF-β. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test.
Where *p˂ .05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.Figure 3 showed the effect of the
β-sitosterol-SLN on cytokine levels of experimental rats tissue. CFA induced rats showed
the increased level of TNF-α (74.95 ± 2.34 pg/mg), IL-1β (55.5 ± 2.04 pg/mg), IL-2
(84.5 ± 2.94 pg/mg), IL-6 (22.43 ± 1.93 pg/mg), IL-16 (33.43 ± 2.09 pg/mg), IL-17
(86.85 ± 3.05 pg/mg) and reduced the IL-10 (7.5 ± 0.94 pg/mg), TGF-β (15.2 ± 1.47 pg/mg)
as compared to normal rats and β-sitosterol-SLN significantly (p <.001) reduced the TNF-α (23.41 ± 1.97 pg/mg), IL-1β
(8.12 ± 0.74 pg/mg), IL-6 (12.03 ± 0.91 pg/mg), IL-2 (16.5 ± 1.84 pg/mg), IL-16
(12.3 ± 1.93 pg/mg), IL-1β (18.54 ± 3.94 pg/mg), IL-17 (17.34 ± 2.04 pg/mg) and
increased the IL-10 (21.43 ± 1.82 pg/mg), TGF-β (57.65 ± 3.46 pg/mg) as compared to CFA
control rats.
Figure 3.
The effect of β-sitosterol-SLNs on cytokines level (tissue) of CFA induced rats.
a: TNF-α, b: Il-6, c: IL-10,
d: IL-2, e: IL-1β, f: IL-16,
g: IL-17 and h: TGF-β. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test.
Where *p˂ .05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
The effect of β-sitosterol-SLNs on cytokines level (tissue) of CFA induced rats.
a: TNF-α, b: Il-6, c: IL-10,
d: IL-2, e: IL-1β, f: IL-16,
g: IL-17 and h: TGF-β. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test.
Where *p˂ .05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
Effect of β-sitosterol-SLN on inflammatory mediators
Figure 4 demonstrated the effect of
β-sitosterol-SLN on the inflammatory mediator of experimental rats serum. CFA-induced
rats showed the increased level of NF-κB (198.34 ± 4.56 pg/ml), PGE2
(80.64 ± 2.91 pg/ml), COX-2 (79.03 ± 3.84 pg/ml), VEGF (53.95 ± 2.90 pg/ml) as compared
to control group rats. β-sitosterol-SLN significantly (p < .001) decreased the level of NF-κB (45.67 ± 2.05 pg/ml),
PGE2 (22.41 ± 1.03 pg/ml), COX-2 (25.41 ± 1.48 pg/ml), VEGF
(11.68 ± 1.14 pg/ml) as compared to CFA control group rats.
Figure 4.
The effect of β-sitosterol-SLNs on inflammatory parameter (Serum) of CFA induced
rats. a: NF-κB, b: PGE2, c: COX-2
and d: VEGF. All the data presented ± SEM. Statistical analysis was
performed via One-way ANOVA followed by Dennett’s test. Where *p˂.05 is significant, **p < .01 is more
significant and ***p < .001 is extreme
significant.
The effect of β-sitosterol-SLNs on inflammatory parameter (Serum) of CFA induced
rats. a: NF-κB, b: PGE2, c: COX-2
and d: VEGF. All the data presented ± SEM. Statistical analysis was
performed via One-way ANOVA followed by Dennett’s test. Where *p˂.05 is significant, **p < .01 is more
significant and ***p < .001 is extreme
significant.Figure 5 demonstrated the effect of
β-sitosterol-SLN on the inflammatory mediator of experimental rats serum. CFA induced
rats showed the increased level of NF-κB (1.98 ± 0.58 pg/mg), PGE2
(1.78 ± 0.74 pg/mg), COX-2 (1.76 ± 0.71 pg/mg), VEGF (0.58 ± 0.15 pg/mg) as compared to
control group rats. β-sitosterol-SLN significantly (p < .001) decreased the level of NF-κB (0.42 ± 0.12 pg/mg), PGE2
(0.31 ± 0.09 pg/mg), COX-2 (0.28 ± 0.3 pg/mg), VEGF (0.18 ± 0.03 pg/mg) as compared to
CFA control group rats.
Figure 5.
The effect of β-sitosterol-SLNs on inflammatory parameter (tissue) of CFA induced
rats. a: NF-κB, b: PGE2, c: COX-2
and d: VEGF. All the data presented ± SEM. Statistical analysis was
performed via One-way ANOVA followed by Dennett’s test. Where *p˂.05 is significant, **p < .01 is more
significant and *** p < .001 is extreme
significant.
The effect of β-sitosterol-SLNs on inflammatory parameter (tissue) of CFA induced
rats. a: NF-κB, b: PGE2, c: COX-2
and d: VEGF. All the data presented ± SEM. Statistical analysis was
performed via One-way ANOVA followed by Dennett’s test. Where *p˂.05 is significant, **p < .01 is more
significant and *** p < .001 is extreme
significant.
Effect of β-sitosterol-SLN on HIF1α and ANG-1
During the arthritis, boosted the level of HIF1α and ANG-1, a similar result was
obtained in the CFA group rats. β-sitosterol-SLN significantly (P < 0.001) reduced the level of HIF1α and ANG-1 as compared to other
groups. β-sitosterol (2.5 and 25 mg/kg) and indomethacin treated group rats showed the
significantly suppression of the level of HIF1α and ANG-1 (Figure 6).
Figure 6.
The effect of β-sitosterol-SLNs on HIF1α and ANG-1 parameter of CFA induced rats.
a: HIF1α and b: ANG-1. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test.
Where *p˂.05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
The effect of β-sitosterol-SLNs on HIF1α and ANG-1 parameter of CFA induced rats.
a: HIF1α and b: ANG-1. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test.
Where *p˂.05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
Quantitative RT-PCR gene expression
Figure 7 showed the effect of β-sitosterol-SLN on
the different gene expression. CFA induced rats showed the increased expression of NF-κB,
HO-1 and reduced expression of Nrf2. β-sitosterol-SLN significantly (p < .001) suppressed the expression of NF-κB, HO-1 and boosted the
expression of HO-1.
Figure 7.
The effect of β-sitosterol-SLNs on mRNA expression (HO-1, Nrf2 and NF-κB)
of CFA induced rats. a: HO-1, b: Nrf2 and
c: NF-κB. All the data presented ± SEM. Statistical analysis was
performed via One-way ANOVA followed by Dennett’s test. Where *p˂.05 is significant, **p < .01 is more
significant and ***p < .001 is extreme
significant.
The effect of β-sitosterol-SLNs on mRNA expression (HO-1, Nrf2 and NF-κB)
of CFA induced rats. a: HO-1, b: Nrf2 and
c: NF-κB. All the data presented ± SEM. Statistical analysis was
performed via One-way ANOVA followed by Dennett’s test. Where *p˂.05 is significant, **p < .01 is more
significant and ***p < .001 is extreme
significant.Figure 8 demonstrated the expression of RANKL and
STAT-3. CFA induced rats showed the increased expression of RANKL and STAT-3.
β-sitosterol-SLN significantly (p < .001) reduced the
expression of RANKL and STAT-3.
Figure 8.
The effect of β-sitosterol-SLNs on RANKL and STAT-3 expression of CFA induced rats.
a: RANKL and b: STAT-3. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test. Where
*p˂.05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
The effect of β-sitosterol-SLNs on RANKL and STAT-3 expression of CFA induced rats.
a: RANKL and b: STAT-3. All the data presented ± SEM.
Statistical analysis was performed via One-way ANOVA followed by Dennett’s test. Where
*p˂.05 is significant, **p < .01 is more significant and ***p < .001 is extreme significant.
Discussion
SLNs provide a novel deliver physicochemically compromised and poorly permeable drug across
the gastrointestinal (GI) mucosa, resulting considerably enhanced the plasma concentration
(Arora et al., 2015). Nano-sized and subsequently
enhanced the surface area of nanoparticles may show the high bio-adhesion to the GI wall,
ensuring the higher, effective and prolonged uptake β-sitosterol embedded in the SLN's solid
lipid matrix is expected to be protected against enzymatic degradation, both in the gut and
through the liver. Surfactant and co-surfactant used in the preparation of β-sitosterol-SLNs
contributed to their increased permeability across the intestinal membrane. Although free
β-sitosterol undergoes for first pass metabolism, SLNs are allegedly lymphatically absorbed
which further bypass the 1st pass circulation via liver for orally administration (Arora
et al., 2015). Particle of size < 200 trend to
bypass reticuloendothelial system pickup via spleen and liver, thereby avoiding liver (major
site of drug degradation and metabolism of β-sitosterol). Thus, β-sitosterol-SLNs (146.7 nm)
will remain in circulation for prolonged periods, achieve prolonged high blood levels and
decrease clearance after absorption. Therefore, enhanced systemic bioavailability
complemented by enhanced penetrability as shown by their preferential distribution into
various tissues such as bones (Thakkar et al., 2007) may obvious itself in achieving higher concentration in the joint synovium,
showing higher anti-inflammatory response in CFA-inflamed joints.Rheumatoid, symptom like deformity, swelling in the ankle or joint, systemic change and
release of autoantibody is an autoimmune disease categorized via generation of chronic
inflammation in the synovial joint (Kumar et al., 2015a, 2016b). During RA condition,
expansion of swelling of the synovium due to the proliferation of synovial cells and take
part in the cartilage deterioration. Prolonged inflammation during the RA, linked with the
bone erosion and affected 80% of patients and occurs rapidly. Additionally, the misbalance
in the immune functions especially reflects the imbalance between the humoral immunity and
cellular immunity. Research suggest that the cellular immunity activated the T1 cells, thus
start the secretion of pro-inflammatory cytokines and humoral immunity reduced the secretion
of T2 inflammatory cytokines (Rahman et al., 2017). Previous studies suggest that the production of cytokines start in the
lymphocytes in the synovium and mononuclear macrophages and play a crucial role in the
pathogenesis of RA. Though cytokines have a critical role in the persistence of RA disease
(Kumar et al., 2015a; Rahman et al., 2015, 2017).The CFA-induced arthritis model is commonly used to analyze the anti-arthritis potential of
the drugs tested. Inspired by the clarification of β-sitosterol-SLN's anti-inflammatory
ability and to explore its long-term anti-inflammatory effects (Kumar et al., 2015a, c). In this experimental study, the
β-sitosterol-SLN was then evaluated against arthritis induced by the adjuvant-induced
immunological chronic inflammation, especially complete Fruend adjuvant (CFA). That causes
common humanarthritis and is more common to pathological and clinical circumstances.
Previous work indicates that adjuvant initiates the secretion of inflammatory mediators and
stimulates irritated phagocytes that play a major role in fibrosis, vascular and tissue
degradation over time (Kumar et al., 2015a, c).
After injecting the adjuvant into the rat, in the first phase start the swelling into the
hind paw and progressively increased (which continued for next few weeks) and after the few
week, adjuvant start the accumulation into the soft tissue of rat and expand the nodules in
tail, ear contralateral part and front paw of experimental rats (Kumar et al., 2015a, c, 2016b). β-sitosterol-SLN significantly reduced the humoral immune reaction due to
suppression the acute inflammation via down-regulating the vascular permeability and
inhibiting the pro-inflammatory cytokines. Adjuvant develops the secondary reaction after
the 2 weeks and significantly reduced by β-sitosterol-SLN. Apparently, CFA-induced secondary
lesions were exposed to delayed hypersensitivity reactions and β-sitosterol-SLN also had an
apparent effect on this, showing its antiarthritic effect.Arthritic rats induced by CFA demonstrated the reduced body weight until the end of the
experimental test (28 days). Previous research indicates that the decreased body weight
observed in CFA mediated group rats due to a lack of leucine and glucose absorption by the
intestines (Kumar et al., 2015a, c, 2016b, a). β-sitosterol-SLN significantly (p < .001) increased the body weight via increase the absorption
of leucine and glucose via intestine.Previous research suggests that during the arthritic condition, the level of Hb, RBC was
reduced and WBC, ECR level was increased. Arthritic condition, the level of RBC reduced and
produced the animatic condition due to erythrocyte deformability (shorten life span of
erythrocytes) (Aiyalu et al., 2016; Mahdi et al.,
2018). Another hematological parameter such as
Hb, reduced observed during the arthritic condition, resultant suppression of bone marrow
erythropoietin and destruction of premature RBCs (Patil et al., 2011; Premaratna et al., 2011). β-sitosterol-SLN significantly (P < 0.001)
restored the level of RBC and Hb near the normal level and support the anti-arthritic effect
of β-sitosterol-SLN. WBC is an important component of the immune system linked to the
induction of an inflammatory reaction and its associated other diseases (Aiyalu et al.,
2016; Kumar et al., 2016b). Clinical study suggests that IL-1β increased the level of WBC
and start the production of inflammatory component like granulocyte and macrophages and also
induce the growth of colony stimulating factors (Kim and Park 2006). CFA-induced arthritic rats treated with β-sitosterol-SLN
significantly (p < 0.001) reduced the migration of
inflammatory granulocytes and macrophage. Another hematological component, ESR, begins the
production of endogenous proteins such as α/β globulin and fibrinogen and suggests arthritic
disease progression (Kumar et al., 2016b).Research suggests that reactive oxygen species (ROS)/reactive nitrogen species (RNS) are
generated in normal cellular metabolism inside the body and play an important role in
attacking the microbial agent. Any disparity between ROS/RNS production and inactivation
leads to cellular dysfunction and unwanted condition of inflammatory diseases such as
arthritis. As we know, that these ROS having the damaging property, body has developed
numerous antioxidant mechanism to prevent the ROS induced damage. During the arthritic
condition, enhanced the ROS synthesis via activated the neutrophils and phagocyte during the
oxidative rush, which cross the limit of endogenous antioxidant resultant induce the
oxidative stress. Continuous production or generation of ROS in the synovial membrane
initiates damaging nucleic acid, collagen, lipids and protein, which additionally turns into
signals for the inflammatory cells and deteriorates the condition of arthritic disease.
Research suggests that ROS acts as a stimulating signal to activate the NF-kB pathway,
leading to alterations of different transcription mediators and pro-inflammatory cytokines.
In the current experimental study, immunization with adjuvant resultant in the suppression
the level of endogenous antioxidant like GSH, CAT and SOD and enhancement of pro-oxidant
like TBARS in arthritic rats. β-sitosterol-SLN significantly (P < 0.001) increased the level of endogenous antioxidant like GSH, CAT and
SOD and reduced the level of pro-oxidant like TBARS as compared to arthritic rats.Previous research suggests that during the RA condition, the cytokines divided into 2
groups like one group produced via lymphocytes and secrete the macrophages/monocytes viz.,
TNF-α, IL-1β, IL-6, IL-10, IL-16, IL-17 and IL-18. Previous research also suggests that the
various factors directly or indirectly interact with the cytokines, which further constrain
or boost the incidence and expansion of numerous disease. TNF-α is a well-known cytokines
that affect the various functions implicated in the RA pathogenesis such as accumulating
leukocytes, chemokines, activation chondrocytes and osteoclasts, activated endothelial
cells, endorsing articular dysfunction and nociceptor sensitization (Brennan & McInnes,
2008). TNF-α is the present high amount during
the RA disease and its induce the local joint tissue destruction and other clinical
symptoms. According to Kumar et al., the high amount of TNF-α was found in the RArats and
targeting the TNF-α for relief the RA disease (Kumar et al., 2015a). Previous research suggests that the IL-1β is the essential
factor for the expansion of RA pathology and present in the joint cavity and it can support
the cell migration and enhance the endothelial cells. Targeting the IL-1β is best way to
treat RA disease. Another pro-inflammatory cytokine like IL-16 released from the T
lymphocytes and expand the RA disease. During the RA, IL-16 not only showed the effect on
the cartilage collagen but also reduces the bone synthesis and boosts the osteoclast
differentiation. Another pro-inflammatory cytokine such as IL-6 play a synergetic role with
IL-1β and TNF-α to increase the inflammatory reactions. In the current experimental study,
we scrutiny the role of inflammatory cytokines and lymphocytes in CFA-induced arthritis and
explore the mechanism at cellular and molecular levels. β-sitosterol-SLN significantly
(p < .001) reduced the inflammatory response in the
synovial cavity in the CFA-induced RArats and decrease the arthritic grading of synovitis
via reducing the level of IL-1β, IL-6, IL-16 and TNF-α in the serum of experimental
rats.NF-κB plays an important role in the expansion of arthritis and various researchers
targeting the NF-κB signaling pathway to treat the arthritic disease. NF-κB plays a role in
regulating/circulating the immune-inflammatory response (Brennan & McInnes, 2008; Isomäki, 2012). NF-κB increases the specific genes such as chemokines, cytokines and
histocompatibility complex and receptors that are necessary for the immune cell migration
and adhesion in addition to apoptosis and cellular proliferation. In the synovial biopsy of
animal and human exhibited the over-expression of NF-κB (Kamel et al., 2018). In this study, CFA treated rats showed the increased level of
NF-κB and β-sitosterol-SLN significantly (P < 0.001)
decreased the NF-κB level in the serum and tissue. β-sitosterol-SLN reduced the level of
NF-κB might be due to suppression of significant pro-inflammatory cytokines IL-17. In
support, Kim et al., claimed that β-sitosterol showed the anti-inflammatory effect in high
fat diet induced intestinal inflammation via suppression of NF-κB pathway (Kim et al., 2014).Previous research suggest that the Nrf2 is a significant transcription factor
commonly present to induce the numerous set of antioxidant enzymes like HO-1, GPx and
glutathione S-transferanse, via binding a sequence of DNA called anti-oxidant response
elements (ARE), which reduced the pro-inflammatory pathway and oxidative stress. Previous
animal investigation suggests the potential relation between the NF-kB and Nrf2,
and showed the joint destruction and oxidative stress in rats. CFA induced rats exhibited
the increased expression of HO-1 and Nrf2 and β-sitosterol-SLN significantly (P < 0.001) downregulated the expression of HO-1 and Nrf2. On the
basis of result, we can conclude that β-sitosterol-SLN reduced the pro-inflammatory
cytokines and oxidative stress due to modulating the HO-1/Nrf2 signaling pathway.It is well documented that STAT-3 play an important role in the proliferation during the
RA. STAT-3 is a prime element for TH17 lymphocyte proliferation and fibroblast like
synoviocyte in RA (Krause et al., 2002). CFA
treated rats showed the increased expression of STAT-3 and β-sitosterol significantly
reduced the expression of STAT-3. Previous study suggest that the STAT-3 activate through
IL-6 cytokines and suppressive effect of β-sitosterol-SLN might be due to anti-inflammatory
effect (Zhou et al., 2007). According to the
Kamel et al., STAT-3 is consider as the excellent target for gene therapy during the RA
reported that suppressing STAT-3 funtion induces the synoviocyte apoptosis and converts the
endogenous growth factors include epidermal growth factor into death factors (Kamel et al.,
2018).Angiogenesis, an exciting proliferation of the blood vessels, continually delivers immune
cells (chemotaxis) and cytokines for arthritic lesion development. Angiogenesis, play an
important role in the maintenance and expansion of RA pannus (Paleolog, 1996). VEGF (angiogenic growth factor) is a
significant mediator responsible for the changes at the affected joints via providing oxygen
and nutrients essential for maintaining the proliferation, synoviocyte proliferation,
enhance vascular permeability and persistent nature of arthritic pannus which may start the
swelling in the joint (Paleolog & Miotla, 1998; Bainbridge et al., 2006).
Previous studies suggest that the various factors such as IL-17, TNF-α, Il-6 and ROS are
capable for induction the VEGF (Kamel et al., 2018). Β-sitosterol-SLN significantly inhibited the VEGF level in the serum and
tissue might be due to its anti-inflammatory and antioxidant effect. In support, it was
showed that β-sitosterol is an effectual VEGF suppressor in rat model of renal
carcinogenesis (Sharmila & Sindhu 2017).
Conclusion
The current investigation showed the development of optimized β-sitosterol-SLNs which
showed the satisfactory loading capability, entrapment efficiency, particle size
distribution and invitro release characteristics.
β-sitosterol-SLNs exerted anti-arthritic effect probably due to its anti-inflammatory and
anti-oxidant effect. It is plausible due to directly related to the reduction the cytokines
and inflammatory mediators, suppression the fundamental gene such as STAT-3 as well as
scavenges ROS.Click here for additional data file.Click here for additional data file.
Authors: Anna Rita Bilia; Vieri Piazzini; Clizia Guccione; Laura Risaliti; Martina Asprea; Giada Capecchi; Maria Camilla Bergonzi Journal: Planta Med Date: 2017-02-08 Impact factor: 3.352
Authors: Sunil S Jalalpure; Yuvaraj D Mandavkar; Pallavi R Khalure; Gulab S Shinde; Pournima A Shelar; Amol S Shah Journal: J Ethnopharmacol Date: 2011-10-01 Impact factor: 4.360
Authors: Trent M Woodruff; Anna J Strachan; Nathan Dryburgh; Ian A Shiels; Robert C Reid; David P Fairlie; Stephen M Taylor Journal: Arthritis Rheum Date: 2002-09
Authors: Harith Jameel Mahdi; Nurzalina Abdul Karim Khan; Mohd Zaini Bin Asmawi; Roziahanim Mahmud; Vikneswaran A/L Murugaiyah Journal: Integr Med Res Date: 2017-12-23
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