Multifocal multiphoton excitation and time correlated single photon counting detection for 3-D fluorescence lifetime imaging.

S Kumar; C Dunsby; P A A De Beule; D M Owen; U Anand; P M P Lanigan; R K P Benninger; D M Davis; M A A Neil; P Anand; C Benham; A Naylor; P M W French

Multifocal multiphoton excitation and time correlated single photon counting detection for 3-D fluorescence lifetime imaging.

S Kumar, C Dunsby, P A A De Beule, D M Owen, U Anand, P M P Lanigan, R K P Benninger, D M Davis, M A A Neil, P Anand, C Benham, A Naylor, P M W French

Research output: Contribution to journal › Article › peer-review

Abstract

We report a multifocal multiphoton time-correlated single photon counting (TCSPC) fluorescence lifetime imaging (FLIM) microscope system that uses a 16 channel multi-anode PMT detector. Multiphoton excitation minimizes out-of-focus photobleaching, multifocal excitation reduces non-linear in-plane photobleaching effects and TCSPC electronics provide photon-efficient detection of the fluorescence decay profile. TCSPC detection is less prone to bleaching- and movement-induced artefacts compared to wide-field time-gated or frequency-domain FLIM. This microscope is therefore capable of acquiring 3-D FLIM images at significantly increased speeds compared to single beam multiphoton microscopy and we demonstrate this with live cells expressing a GFP tagged protein. We also apply this system to time-lapse FLIM of NAD(P)H autofluorescence in single live cells and report measurements on the change in the fluorescence decay profile following the application of a known metabolic inhibitor.

Original language	English
Journal	Optics Express
Volume	15
Issue number	20
Publication status	Published - 1 Oct 2007

Cite this

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title = "Multifocal multiphoton excitation and time correlated single photon counting detection for 3-D fluorescence lifetime imaging.",

abstract = "We report a multifocal multiphoton time-correlated single photon counting (TCSPC) fluorescence lifetime imaging (FLIM) microscope system that uses a 16 channel multi-anode PMT detector. Multiphoton excitation minimizes out-of-focus photobleaching, multifocal excitation reduces non-linear in-plane photobleaching effects and TCSPC electronics provide photon-efficient detection of the fluorescence decay profile. TCSPC detection is less prone to bleaching- and movement-induced artefacts compared to wide-field time-gated or frequency-domain FLIM. This microscope is therefore capable of acquiring 3-D FLIM images at significantly increased speeds compared to single beam multiphoton microscopy and we demonstrate this with live cells expressing a GFP tagged protein. We also apply this system to time-lapse FLIM of NAD(P)H autofluorescence in single live cells and report measurements on the change in the fluorescence decay profile following the application of a known metabolic inhibitor.",

author = "S Kumar and C Dunsby and {De Beule}, {P A A} and Owen, {D M} and U Anand and Lanigan, {P M P} and Benninger, {R K P} and Davis, {D M} and Neil, {M A A} and P Anand and C Benham and A Naylor and French, {P M W}",

year = "2007",

month = oct,

day = "1",

language = "English",

volume = "15",

journal = "Optics Express",

publisher = "Optical Society of America",

number = "20",

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TY - JOUR

T1 - Multifocal multiphoton excitation and time correlated single photon counting detection for 3-D fluorescence lifetime imaging.

AU - Kumar, S

AU - Dunsby, C

AU - De Beule, P A A

AU - Owen, D M

AU - Anand, U

AU - Lanigan, P M P

AU - Benninger, R K P

AU - Davis, D M

AU - Neil, M A A

AU - Anand, P

AU - Benham, C

AU - Naylor, A

AU - French, P M W

PY - 2007/10/1

Y1 - 2007/10/1

N2 - We report a multifocal multiphoton time-correlated single photon counting (TCSPC) fluorescence lifetime imaging (FLIM) microscope system that uses a 16 channel multi-anode PMT detector. Multiphoton excitation minimizes out-of-focus photobleaching, multifocal excitation reduces non-linear in-plane photobleaching effects and TCSPC electronics provide photon-efficient detection of the fluorescence decay profile. TCSPC detection is less prone to bleaching- and movement-induced artefacts compared to wide-field time-gated or frequency-domain FLIM. This microscope is therefore capable of acquiring 3-D FLIM images at significantly increased speeds compared to single beam multiphoton microscopy and we demonstrate this with live cells expressing a GFP tagged protein. We also apply this system to time-lapse FLIM of NAD(P)H autofluorescence in single live cells and report measurements on the change in the fluorescence decay profile following the application of a known metabolic inhibitor.

AB - We report a multifocal multiphoton time-correlated single photon counting (TCSPC) fluorescence lifetime imaging (FLIM) microscope system that uses a 16 channel multi-anode PMT detector. Multiphoton excitation minimizes out-of-focus photobleaching, multifocal excitation reduces non-linear in-plane photobleaching effects and TCSPC electronics provide photon-efficient detection of the fluorescence decay profile. TCSPC detection is less prone to bleaching- and movement-induced artefacts compared to wide-field time-gated or frequency-domain FLIM. This microscope is therefore capable of acquiring 3-D FLIM images at significantly increased speeds compared to single beam multiphoton microscopy and we demonstrate this with live cells expressing a GFP tagged protein. We also apply this system to time-lapse FLIM of NAD(P)H autofluorescence in single live cells and report measurements on the change in the fluorescence decay profile following the application of a known metabolic inhibitor.

M3 - Article

C2 - 19550524

VL - 15

JO - Optics Express

JF - Optics Express

IS - 20

ER -

Multifocal multiphoton excitation and time correlated single photon counting detection for 3-D fluorescence lifetime imaging.

Abstract

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