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Literature DB >> 21808026

Phasor approach to fluorescence lifetime microscopy distinguishes different metabolic states of germ cells in a live tissue.

Chiara Stringari¹, Amanda Cinquin, Olivier Cinquin, Michelle A Digman, Peter J Donovan, Enrico Gratton.

Abstract

We describe a label-free imaging method to monitor stem-cell metabolism that discriminates different states of stem cells as they differentiate in living tissues. In this method we use intrinsic fluorescence biomarkers and the phasor approach to fluorescence lifetime imaging microscopy in conjunction with image segmentation, which we use to introduce the concept of the cell phasor. In live tissues we are able to identify intrinsic fluorophores, such as collagen, retinol, retinoic acid, porphyrin, flavins, and free and bound NADH. We have exploited the cell phasor approach to detect a trend in metabolite concentrations along the main axis of the Caenorhabditis elegans germ line. This trend is consistent with known changes in metabolic states during differentiation. The cell phasor approach to lifetime imaging provides a label-free, fit-free, and sensitive method to identify different metabolic states of cells during differentiation, to sense small changes in the redox state of cells, and may identify symmetric and asymmetric divisions and predict cell fate. Our method is a promising noninvasive optical tool for monitoring metabolic pathways during differentiation or disease progression, and for cell sorting in unlabeled tissues.

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Year: 2011 PMID： 21808026 PMCID： PMC3158156 DOI： 10.1073/pnas.1108161108

Source DB: PubMed Journal: Proc Natl Acad Sci U S A ISSN： 0027-8424 Impact factor: 11.205

47 in total

Review 1. Extrinsic regulation of pluripotent stem cells.

Authors: Martin F Pera; Patrick P L Tam
Journal: Nature Date: 2010-06-10 Impact factor: 49.962

2. Live tissue intrinsic emission microscopy using multiphoton-excited native fluorescence and second harmonic generation.

Authors: Warren R Zipfel; Rebecca M Williams; Richard Christie; Alexander Yu Nikitin; Bradley T Hyman; Watt W Webb
Journal: Proc Natl Acad Sci U S A Date: 2003-05-19 Impact factor: 11.205

Review 3. Deep tissue two-photon microscopy.

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

4. In vivo multiphoton microscopy of NADH and FAD redox states, fluorescence lifetimes, and cellular morphology in precancerous epithelia.

Authors: Melissa C Skala; Kristin M Riching; Annette Gendron-Fitzpatrick; Jens Eickhoff; Kevin W Eliceiri; John G White; Nirmala Ramanujam
Journal: Proc Natl Acad Sci U S A Date: 2007-11-27 Impact factor: 11.205

Review 5. Caenorhabditis elegans germ line: a model for stem cell biology.

Authors: E Jane Albert Hubbard
Journal: Dev Dyn Date: 2007-12 Impact factor: 3.780

6. Time-correlated single photon counting FLIM: some considerations for physiologists.

Authors: Claire N Medine; Angela McDonald; Axel Bergmann; Rory R Duncan
Journal: Microsc Res Tech Date: 2007-05 Impact factor: 2.769

7. Fluorescence lifetime imaging of free and protein-bound NADH.

Authors: J R Lakowicz; H Szmacinski; K Nowaczyk; M L Johnson
Journal: Proc Natl Acad Sci U S A Date: 1992-02-15 Impact factor: 11.205

8. Multiphoton fluorescence lifetime imaging of intrinsic fluorescence in human and rat brain tissue reveals spatially distinct NADH binding.

Authors: Thomas H Chia; Anne Williamson; Dennis D Spencer; Michael J Levene
Journal: Opt Express Date: 2008-03-17 Impact factor: 3.894

9. Cellular analyses of the mitotic region in the Caenorhabditis elegans adult germ line.

Authors: Sarah L Crittenden; Kimberly A Leonhard; Dana T Byrd; Judith Kimble
Journal: Mol Biol Cell Date: 2006-05-03 Impact factor: 4.138

Review 10. Purpose and regulation of stem cells: a systems-biology view from the Caenorhabditis elegans germ line.

Authors: Olivier Cinquin
Journal: J Pathol Date: 2009-01 Impact factor: 7.996

156 in total

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Authors: Xiaolu A Cambronne; W Lee Kraus
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2. Enhancing spontaneous emission rates of molecules using nanopatterned multilayer hyperbolic metamaterials.

Authors: Dylan Lu; Jimmy J Kan; Eric E Fullerton; Zhaowei Liu
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Review 3. Cell metabolomics.

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4. Simultaneous imaging of two-photon absorption and stimulated Raman scattering by spatial overlap modulation nonlinear optical microscopy.

Authors: Keisuke Isobe; Hiroyuki Kawano; Akira Suda; Akiko Kumagai; Atsushi Miyawaki; Katsumi Midorikawa
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5. Inhibition of 5-lipoxygenase decreases renal fibrosis and progression of chronic kidney disease.

Authors: John R Montford; Colin Bauer; Evgenia Dobrinskikh; Katharina Hopp; Moshe Levi; Mary Weiser-Evans; Raphael Nemenoff; Seth B Furgeson
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6. Targeting cancer metabolism by simultaneously disrupting parallel nutrient access pathways.

Authors: Seong M Kim; Saurabh G Roy; Bin Chen; Tiffany M Nguyen; Ryan J McMonigle; Alison N McCracken; Yanling Zhang; Satoshi Kofuji; Jue Hou; Elizabeth Selwan; Brendan T Finicle; Tricia T Nguyen; Archna Ravi; Manuel U Ramirez; Tim Wiher; Garret G Guenther; Mari Kono; Atsuo T Sasaki; Lois S Weisman; Eric O Potma; Bruce J Tromberg; Robert A Edwards; Stephen Hanessian; Aimee L Edinger
Journal: J Clin Invest Date: 2016-09-26 Impact factor: 14.808

Phasor approach to fluorescence lifetime microscopy distinguishes different metabolic states of germ cells in a live tissue.

Review 1. Extrinsic regulation of pluripotent stem cells.

2. Live tissue intrinsic emission microscopy using multiphoton-excited native fluorescence and second harmonic generation.

Review 3. Deep tissue two-photon microscopy.

4. In vivo multiphoton microscopy of NADH and FAD redox states, fluorescence lifetimes, and cellular morphology in precancerous epithelia.

Review 5. Caenorhabditis elegans germ line: a model for stem cell biology.

6. Time-correlated single photon counting FLIM: some considerations for physiologists.

7. Fluorescence lifetime imaging of free and protein-bound NADH.

8. Multiphoton fluorescence lifetime imaging of intrinsic fluorescence in human and rat brain tissue reveals spatially distinct NADH binding.

9. Cellular analyses of the mitotic region in the Caenorhabditis elegans adult germ line.

Review 10. Purpose and regulation of stem cells: a systems-biology view from the Caenorhabditis elegans germ line.

Review 1. Location, Location, Location: Compartmentalization of NAD⁺ Synthesis and Functions in Mammalian Cells.

2. Enhancing spontaneous emission rates of molecules using nanopatterned multilayer hyperbolic metamaterials.

Review 3. Cell metabolomics.

4. Simultaneous imaging of two-photon absorption and stimulated Raman scattering by spatial overlap modulation nonlinear optical microscopy.

5. Inhibition of 5-lipoxygenase decreases renal fibrosis and progression of chronic kidney disease.

6. Targeting cancer metabolism by simultaneously disrupting parallel nutrient access pathways.

7. Application of phasor plot and autofluorescence correction for study of heterogeneous cell population.

8. Intravital microscopy of biosensor activities and intrinsic metabolic states.

9. Spectral Phasor approach for fingerprinting of photo-activatable fluorescent proteins Dronpa, Kaede and KikGR.

10. Structural mapping of fluorescently-tagged, functional nhTMEM16 scramblase in a lipid bilayer.

Review 1. Extrinsic regulation of pluripotent stem cells.

Review 3. Deep tissue two-photon microscopy.

Review 5. Caenorhabditis elegans germ line: a model for stem cell biology.

Review 10. Purpose and regulation of stem cells: a systems-biology view from the Caenorhabditis elegans germ line.

Review 1. Location, Location, Location: Compartmentalization of NAD+ Synthesis and Functions in Mammalian Cells.

Review 3. Cell metabolomics.

Review 1. Location, Location, Location: Compartmentalization of NAD⁺ Synthesis and Functions in Mammalian Cells.