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Literature DB >> 22385865

Excitation spectra and brightness optimization of two-photon excited probes.

Jörg Mütze¹, Vijay Iyer, John J Macklin, Jennifer Colonell, Bill Karsh, Zdeněk Petrášek, Petra Schwille, Loren L Looger, Luke D Lavis, Timothy D Harris.

Abstract

Two-photon probe excitation data are commonly presented as absorption cross section or molecular brightness (the detected fluorescence rate per molecule). We report two-photon molecular brightness spectra for a diverse set of organic and genetically encoded probes with an automated spectroscopic system based on fluorescence correlation spectroscopy. The two-photon action cross section can be extracted from molecular brightness measurements at low excitation intensities, while peak molecular brightness (the maximum molecular brightness with increasing excitation intensity) is measured at higher intensities at which probe photophysical effects become significant. The spectral shape of these two parameters was similar across all dye families tested. Peak molecular brightness spectra, which can be obtained rapidly and with reduced experimental complexity, can thus serve as a first-order approximation to cross-section spectra in determining optimal wavelengths for two-photon excitation, while providing additional information pertaining to probe photostability. The data shown should assist in probe choice and experimental design for multiphoton microscopy studies. Further, we show that, by the addition of a passive pulse splitter, nonlinear bleaching can be reduced--resulting in an enhancement of the fluorescence signal in fluorescence correlation spectroscopy by a factor of two. This increase in fluorescence signal, together with the observed resemblance of action cross section and peak brightness spectra, suggests higher-order photobleaching pathways for two-photon excitation. Copyright Â

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Year: 2012 PMID： 22385865 PMCID： PMC3283774 DOI： 10.1016/j.bpj.2011.12.056

Source DB: PubMed Journal: Biophys J ISSN： 0006-3495 Impact factor: 4.033

31 in total

1. Two-photon imaging in living brain slices.

Authors: Z F Mainen; M Maletic-Savatic; S H Shi; Y Hayashi; R Malinow; K Svoboda
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Review 2. Deep tissue two-photon microscopy.

Authors: Fritjof Helmchen; Winfried Denk
Journal: Nat Methods Date: 2005-12 Impact factor: 28.547

3. Strategies to improve photostabilities in ultrasensitive fluorescence spectroscopy.

Authors: Jerker Widengren; Andriy Chmyrov; Christian Eggeling; Per-Ake Löfdahl; Claus A M Seidel
Journal: J Phys Chem A Date: 2007-01-25 Impact factor: 2.781

4. Ultrafast measurement of two-photon absorption by loss modulation.

Authors: Peifang Tian; Warren S Warren
Journal: Opt Lett Date: 2002-09-15 Impact factor: 3.776

5. Two-Photon Fluorescence Excitation Cross Sections of Biomolecular Probes from 690 to 960 nm.

Authors: M A Albota; C Xu; W W Webb
Journal: Appl Opt Date: 1998-11-01 Impact factor: 1.980

6. Photobleaching in two-photon scanning fluorescence correlation spectroscopy.

Authors: Zdenek Petrásek; Petra Schwille
Journal: Chemphyschem Date: 2008-01-11 Impact factor: 3.102

7. Two-photon laser scanning fluorescence microscopy.

Authors: W Denk; J H Strickler; W W Webb
Journal: Science Date: 1990-04-06 Impact factor: 47.728

8. Imaging cellular signals in the heart in vivo: Cardiac expression of the high-signal Ca2+ indicator GCaMP2.

Authors: Yvonne N Tallini; Masamichi Ohkura; Bum-Rak Choi; Guangju Ji; Keiji Imoto; Robert Doran; Jane Lee; Patricia Plan; Jason Wilson; Hong-Bo Xin; Atsushi Sanbe; James Gulick; John Mathai; Jeffrey Robbins; Guy Salama; Junichi Nakai; Michael I Kotlikoff
Journal: Proc Natl Acad Sci U S A Date: 2006-03-13 Impact factor: 11.205

9. Water-soluble quantum dots for multiphoton fluorescence imaging in vivo.

Authors: Daniel R Larson; Warren R Zipfel; Rebecca M Williams; Stephen W Clark; Marcel P Bruchez; Frank W Wise; Watt W Webb
Journal: Science Date: 2003-05-30 Impact factor: 47.728

10. Absolute measurement of molecular two-photon absorption cross-sections using a fluorescence saturation technique.

Authors: Martin Kauert; Patrick C Stoller; Martin Frenz; Jaro Ricka
Journal: Opt Express Date: 2006-09-04 Impact factor: 3.894

37 in total

1. A structural and genotypic scaffold underlying temporal integration.

Authors: Melanie M Lee; Aristides B Arrenberg; Emre R F Aksay
Journal: J Neurosci Date: 2015-05-20 Impact factor: 6.167

2. Measurements of multiphoton action cross sections for multiphoton microscopy.

Authors: Li-Chung Cheng; Nicholas G Horton; Ke Wang; Shean-Jen Chen; Chris Xu
Journal: Biomed Opt Express Date: 2014-09-04 Impact factor: 3.732

3. Voltage-sensitive rhodol with enhanced two-photon brightness.

Authors: Rishikesh U Kulkarni; Daniel J Kramer; Narges Pourmandi; Kaveh Karbasi; Helen S Bateup; Evan W Miller
Journal: Proc Natl Acad Sci U S A Date: 2017-02-27 Impact factor: 11.205

Review 4. In vivo deep two-photon imaging of neural circuits with the fluorescent Ca²⁺ indicator Cal-590.

Authors: Carsten H Tischbirek; Antje Birkner; Arthur Konnerth
Journal: J Physiol Date: 2017-02-05 Impact factor: 5.182

5. High-accuracy reference standards for two-photon absorption in the 680-1050 nm wavelength range.

Authors: Sophie de Reguardati; Juri Pahapill; Alexander Mikhailov; Yuriy Stepanenko; Aleksander Rebane
Journal: Opt Express Date: 2016-04-18 Impact factor: 3.894

6. Imaging Ca²⁺ with a Fluorescent Rhodol.

Authors: Alisha A Contractor; Evan W Miller
Journal: Biochemistry Date: 2017-11-28 Impact factor: 3.162

7. Efficient non-degenerate two-photon excitation for fluorescence microscopy.

Authors: Sanaz Sadegh; Mu-Han Yang; Christopher G L Ferri; Martin Thunemann; Payam A Saisan; Zhe Wei; Erik A Rodriguez; Stephen R Adams; Kivilcim Kiliç; David A Boas; Sava Sakadžić; Anna Devor; Yeshaiahu Fainman
Journal: Opt Express Date: 2019-09-30 Impact factor: 3.894

Excitation spectra and brightness optimization of two-photon excited probes.

1. Two-photon imaging in living brain slices.

Review 2. Deep tissue two-photon microscopy.

3. Strategies to improve photostabilities in ultrasensitive fluorescence spectroscopy.

4. Ultrafast measurement of two-photon absorption by loss modulation.

5. Two-Photon Fluorescence Excitation Cross Sections of Biomolecular Probes from 690 to 960 nm.

6. Photobleaching in two-photon scanning fluorescence correlation spectroscopy.

7. Two-photon laser scanning fluorescence microscopy.

8. Imaging cellular signals in the heart in vivo: Cardiac expression of the high-signal Ca2+ indicator GCaMP2.

9. Water-soluble quantum dots for multiphoton fluorescence imaging in vivo.

10. Absolute measurement of molecular two-photon absorption cross-sections using a fluorescence saturation technique.

1. A structural and genotypic scaffold underlying temporal integration.

2. Measurements of multiphoton action cross sections for multiphoton microscopy.

3. Voltage-sensitive rhodol with enhanced two-photon brightness.

Review 4. In vivo deep two-photon imaging of neural circuits with the fluorescent Ca²⁺ indicator Cal-590.

5. High-accuracy reference standards for two-photon absorption in the 680-1050 nm wavelength range.

6. Imaging Ca²⁺ with a Fluorescent Rhodol.

7. Efficient non-degenerate two-photon excitation for fluorescence microscopy.

8. Second Harmonic Generation Spectroscopy of Membrane Probe Dynamics in Gram-Positive Bacteria.

9. Deep Tissue Imaging with Multiphoton Fluorescence Microscopy.

10. Live-Animal Imaging of Renal Function by Multiphoton Microscopy.

Review 2. Deep tissue two-photon microscopy.

Review 4. In vivo deep two-photon imaging of neural circuits with the fluorescent Ca2+ indicator Cal-590.

Review 4. In vivo deep two-photon imaging of neural circuits with the fluorescent Ca²⁺ indicator Cal-590.