Issue 11, 2021
From the journal:

Analyst

Mapping sub-cellular protein aggregates and lipid inclusions using synchrotron ATR-FTIR microspectroscopy

David Hartnell, ORCID logo ab   Ashley Hollings,ab   Anna Maria Ranieri,a   Hum Bahadur Lamichhane,a   Thomas Becker, ORCID logo a   Nicole J. Sylvain,c   Huishu Hou,c   M. Jake Pushie, ORCID logo c   Elizabeth Watkin, ORCID logo d   Keith R. Bambery, ORCID logo e   Mark J. Tobin, ORCID logo e   Michael E. Kelly,c   Massimiliano Massi, ORCID logo a   Jitraporn Vongsvivut ORCID logo e  and  Mark J. Hackett ORCID logo *ab  

* Corresponding authors

a School of Molecular and Life Sciences, Curtin University, Bentley, Western Australia
E-mail: mark.j.hackett@curtin.edu.au

b Curtin Health Innovation Research Institute, Curtin University, Bentley, Western Australia

c Division of Neurosurgery, Department of Surgery, College of Medicine, University of Saskatchewan, Saskatoon, Canada S7N 5E5

d Curtin Medical School, Curtin University, Bentley, Western Australia 6845

e ANSTO – Australian Synchrotron, 800 Blackburn Road, Victoria, 3168, Clayton, Australia

Abstract

Visualising direct biochemical markers of cell physiology and disease pathology at the sub-cellular level is an ongoing challenge in the biological sciences. A suite of microscopies exists to either visualise sub-cellular architecture or to indirectly view biochemical markers (e.g. histochemistry), but further technique developments and innovations are required to increase the range of biochemical parameters that can be imaged directly, in situ, within cells and tissue. Here, we report our continued advancements in the application of synchrotron radiation attenuated total reflectance Fourier transform infrared (SR-ATR-FTIR) microspectroscopy to study sub-cellular biochemistry. Our recent applications demonstrate the much needed capability to map or image directly sub-cellular protein aggregates within degenerating neurons as well as lipid inclusions within bacterial cells. We also characterise the effect of spectral acquisition parameters on speed of data collection and the associated trade-offs between a realistic experimental time frame and spectral/image quality. Specifically, the study highlights that the choice of 8 cm−1 spectral resolutions provide a suitable trade-off between spectral quality and collection time, enabling identification of important spectroscopic markers, while increasing image acquisition by ∼30% (relative to 4 cm−1 spectral resolution). Further, this study explores coupling a focal plane array detector with SR-ATR-FTIR, revealing a modest time improvement in image acquisition time (factor of 2.8). Such information continues to lay the foundation for these spectroscopic methods to be readily available for, and adopted by, the biological science community to facilitate new interdisciplinary endeavours to unravel complex biochemical questions and expand emerging areas of study.

Graphical abstract: Mapping sub-cellular protein aggregates and lipid inclusions using synchrotron ATR-FTIR microspectroscopy

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Article information

DOI
https://doi.org/10.1039/D1AN00136A
Article type
Paper
Submitted
22 Jan 2021
Accepted
07 Mar 2021
First published
22 Mar 2021

Analyst, 2021,146, 3516-3525

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Mapping sub-cellular protein aggregates and lipid inclusions using synchrotron ATR-FTIR microspectroscopy

D. Hartnell, A. Hollings, A. M. Ranieri, H. B. Lamichhane, T. Becker, N. J. Sylvain, H. Hou, M. J. Pushie, E. Watkin, K. R. Bambery, M. J. Tobin, M. E. Kelly, M. Massi, J. Vongsvivut and M. J. Hackett, Analyst, 2021, 146, 3516 DOI: 10.1039/D1AN00136A

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