Silicon nitride as a versatile growth substrate for microspectroscopic imaging and mapping of individual cells

被引:63
作者
Carter, Elizabeth A. [1 ]
Rayner, Benjamin S. [2 ]
McLeod, Andrew I. [1 ]
Wu, Lindsay E. [1 ]
Marshall, Craig P. [1 ]
Levina, Aviva [1 ]
Aitken, Jade B. [1 ]
Witting, Paul K. [2 ]
Lai, Barry [3 ]
Cai, Zhonghou [3 ]
Vogt, Stefan [3 ]
Lee, Yao-Chang [4 ]
Chen, Ching-Iue [4 ]
Tobin, Mark J. [5 ]
Harris, Hugh H. [1 ]
Lay, Peter A. [1 ]
机构
[1] Univ Sydney, Sch Chem, Sydney, NSW 2006, Australia
[2] Concord Repatriat Gen Hosp, ANZAC Res Inst, Concord, NSW 2139, Australia
[3] Argonne Natl Lab, Adv Photon Source, Argonne, IL 60439 USA
[4] Natl Synchrotron Radiat Res Ctr, Hsinchu 30076, Taiwan
[5] Australian Synchrotron, Clayton, Vic 3168, Australia
基金
澳大利亚研究理事会;
关键词
RAMAN-SPECTROSCOPY; INFRARED MICROSPECTROSCOPY; SYNCHROTRON-RADIATION; IR MICROSPECTROSCOPY; FT-IR; DIFFERENTIATION; INSULIN; INJURY; LINE;
D O I
10.1039/c001499k
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Herein is described a general sampling protocol that includes culture, differentiation and. xing of cells in their preferred morphology on the one sample substrate (Si(3)N(4)) to enable subsequent diverse modern microspectroscopic analyses. The protocol enables unprecedented correlated and complementary information on the intracellular biochemistry of metabolic processes, diseases and their treatment, which offers the opportunity to revolutionize our understanding of cell and tissue biology at a molecular level. The culture of adherent cells onto inexpensive Si3N4 membranes allows microspectroscopic analyses across the electromagnetic spectrum, from hard X-ray fluorescence (both XRF and XANES), through to visible and fluorescence light microscopies, and infrared microspectroscopy without substrate interference. Adherent mammalian cell lines (3T3-L1 adipocytes and H9c2 cardiac myocytes) illustrate the in vitro application of these protocols. The cells adhered strongly to Si(3)N(4) membranes and visually displayed normal proliferative and phenotypic growth; more importantly, rapid alcohol fixation of cells did not affect their structural integrity for subsequent analyses.
引用
收藏
页码:1316 / 1322
页数:7
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