PMID- 11823234
OWN - NLM
STAT- MEDLINE
DCOM- 20020328
LR  - 20210526
IS  - 0099-2240 (Print)
IS  - 1098-5336 (Electronic)
IS  - 0099-2240 (Linking)
VI  - 68
IP  - 2
DP  - 2002 Feb
TI  - Assessment of fluorochromes for two-photon laser scanning microscopy of biofilms.
PG  - 901-9
AB  - A major limitation for the use of two-proton laser scanning microscopy (2P-LSM) 
      in biofilm and other studies is the lack of a thorough understanding of the 
      excitation-emission responses of potential fluorochromes. In order to use 2P-LSM, 
      the utility of various fluorochromes and probes specific for a range of biofilm 
      constituents must be evaluated. The fluorochromes tested in this study included 
      classical nucleic acid-specific stains, such as acridine orange (AO) and 
      4",6"-diamidino-2-phenylindole (DAPI), as well as recently developed stains. In 
      addition, stains specific for biofilm extracellular polymeric substances (EPS 
      matrix components) were tested. Two-photon excitation with a Ti/Sapphire laser 
      was carried out at wavelengths from 760 to 900 nm in 10-nm steps. It was found 
      that autofluorescence of phototrophic organisms (cyanobacteria and green algae) 
      resulted in strong signals for the entire excitation range. In addition, the 
      coenzyme F(420)-related autofluorescence of methanogenic bacteria could be used 
      to obtain images of dense aggregates (excitation wavelength, 780 nm). The 
      intensities of the emission signals for the nucleic acid-specific fluorochromes 
      varied. For example, the intensities were similar for excitation wavelengths 
      ranging from 780 to 900 nm for AO but were higher for a narrower range, 780 to 
      810 nm, for DAPI. In selective excitation, fading, multiple staining, and 
      combined single-photon-two-photon studies, the recently developed nucleic 
      acid-specific fluorochromes proved to be more suitable regardless of whether they 
      are intended for living or fixed samples. Probes specific for proteins and 
      glycoconjugates allowed two-photon imaging of polymeric biofilm constituents. 
      Selective excitation-emission was observed for Calcofluor White M2R (780 to 800 
      nm) and SyproOrange (880 to 900 nm). In addition, fluor-conjugated concanavalin A 
      lectins were examined and provided acceptable two-photon emission signals at 
      wavelengths ranging from 780 to 800 nm. Finally, CellTracker, a fluorochrome 
      suitable for long-term labeling of microbial eucaryote cells, was found to give 
      strong emission at wavelengths ranging from 770 to 810 nm. If fluorochromes have 
      the same two-photon excitation cross section, they are suitable for multiple 
      staining and multichannel recording. Generally, if an appropriate excitation 
      wavelength and fluorochrome were used, it was possible to obtain more highly 
      resolved images for thick biofilm samples with two-photon laser microscopy than 
      with conventional single-photon laser microscopy. Due to its potential for higher 
      resolution in light-scattering tissue-like material, such as biofilms, and 
      extremely localized excitation, 2P-LSM is a valuable addition to conventional 
      confocal laser scanning microscopy with single-photon excitation. However, 
      further development of the method and basic research are necessary to take full 
      advantage of nonlinear excitation in studies of interfacial microbial ecology.
FAU - Neu, Thomas R
AU  - Neu TR
AD  - Department of Inland Water Research Magdeburg, UFZ Centre for Environmental 
      Research Leipzig-Halle, Brueckstrasse 3a, 39114 Magdeburg, Germany. neu@gm.ufz.de
FAU - Kuhlicke, Ute
AU  - Kuhlicke U
FAU - Lawrence, John R
AU  - Lawrence JR
LA  - eng
PT  - Evaluation Study
PT  - Journal Article
PL  - United States
TA  - Appl Environ Microbiol
JT  - Applied and environmental microbiology
JID - 7605801
RN  - 0 (Fluorescent Dyes)
SB  - IM
EIN - Appl Environ Microbiol 2002 Apr;68(4):2093
MH  - Biofilms/*growth & development
MH  - Cyanobacteria/*growth & development/metabolism
MH  - Fluorescent Dyes/*metabolism
MH  - Fungi/growth & development/*metabolism
MH  - Microscopy, Confocal/*methods
MH  - *Photons
MH  - Staining and Labeling/methods
PMC - PMC126725
EDAT- 2002/02/02 10:00
MHDA- 2002/03/29 10:01
PMCR- 2002/02/01
CRDT- 2002/02/02 10:00
PHST- 2002/02/02 10:00 [pubmed]
PHST- 2002/03/29 10:01 [medline]
PHST- 2002/02/02 10:00 [entrez]
PHST- 2002/02/01 00:00 [pmc-release]
AID - 1392 [pii]
AID - 10.1128/AEM.68.2.901-909.2002 [doi]
PST - ppublish
SO  - Appl Environ Microbiol. 2002 Feb;68(2):901-9. doi: 10.1128/AEM.68.2.901-909.2002.