Issue 14, 2019
From the journal:

Analyst

Fluorescence imaging of stained red blood cells with simultaneous resonance Raman photostability analysis

Ansam J. Talib, ORCID logo ab   Andrew Fisher, ORCID logo e   Dmitri V. Voronine, ORCID logo *cd   Alexander M. Sinyukov, ORCID logo a   Sandra C. Bustamante Lopez,ae   Sharad Ambardar, ORCID logo cd   Kenith E. Meissner, ORCID logo e   Marlan O. Scullyaf  and  Alexei V. Sokolov ORCID logo af  

* Corresponding authors

a Institute for Quantum Science and Engineering, Texas A&M University, College Station, TX 77843, USA

b Department of Physics, University of Thi-Qar, Thi-Qar, Iraq

c Department of Physics, University of South Florida, Tampa, FL 33620, USA
E-mail: dmitri.voronine@gmail.com

d Department of Medical Engineering, University of South Florida, Tampa, FL 33620, USA

e Department of Physics, Centre for Nanohealth, Swansea University, Swansea, Wales, UK

f Department of Physics, Baylor University, Waco, TX 76706, USA

Abstract

Optical spectroscopic imaging of biological systems has important applications in medical diagnosis, biochemistry, and image-guided surgery. Vibrational spectroscopy, such as Raman scattering, provides high chemical selectivity but is limited by weak signals and a large fluorescence background. Fluorescence imaging is often used by introducing specific dyes in biological systems to label different system parts and to increase the image contrast. However, the extrinsic fluorescence of the staining molecules often masks the intrinsic vibrational signals of biomolecules, which could also be simultaneously detected using the same excitation laser source. Therefore, fluorescence staining is often accompanied by the loss of other important complimentary information. For example, the high laser power often used for the rapid, high-quality imaging could lead to photo-induced suppression or bleaching of the fluorescence and Raman signals resulting in sample photodamage. Therefore, simultaneous imaging and photodamage analysis need to be performed in a controlled bioimaging experiment. Here we perform simultaneous spectroscopic bioimaging and photostability analysis of rhodamine 6G (R6G) stained red blood cells (RBCs) using both fluorescence and resonance Raman imaging in a single 532 nm laser excitation experiment. We develop a corresponding data processing algorithm which allows separation of the two spectroscopic signals. We control the relative intensity of the R6G and RBC signals by varying the excitation laser power and simultaneously monitor the photostability of RBCs. We observe no significant photodamage of RBCs through the absence of changes in the relative Raman peak intensities. Conversely, the R6G molecules show bleaching with the suppression of both the fluorescence and resonance Raman signals. Our approach may be generalized to other types of stained cells with the appropriate selection of fluorescent dyes and excitation sources.

Graphical abstract: Fluorescence imaging of stained red blood cells with simultaneous resonance Raman photostability analysis

About
Cited by
Related
Download options Please wait...

Supplementary files

Article information

DOI
https://doi.org/10.1039/C9AN00757A
Article type
Paper
Submitted
26 Apr 2019
Accepted
05 Jun 2019
First published
07 Jun 2019

Analyst, 2019,144, 4362-4370

Author version available


Download author version (PDF)

Permissions

Request permissions

Fluorescence imaging of stained red blood cells with simultaneous resonance Raman photostability analysis

A. J. Talib, A. Fisher, D. V. Voronine, A. M. Sinyukov, S. C. Bustamante Lopez, S. Ambardar, K. E. Meissner, M. O. Scully and A. V. Sokolov, Analyst, 2019, 144, 4362 DOI: 10.1039/C9AN00757A

To request permission to reproduce material from this article, please go to the Copyright Clearance Center request page.

If you are an author contributing to an RSC publication, you do not need to request permission provided correct acknowledgement is given.

If you are the author of this article, you do not need to request permission to reproduce figures and diagrams provided correct acknowledgement is given. If you want to reproduce the whole article in a third-party publication (excluding your thesis/dissertation for which permission is not required) please go to the Copyright Clearance Center request page.

Read more about how to correctly acknowledge RSC content.

Social activity

Spotlight

Advertisements