Sage Journals: Discover world-class research

Abstract

Usefulness of general-purpose fluorogenic assay kits to determine caspase 3/7 activity of biological extracts is highly compromised in meat-based samples due to their scarce enzyme concentration. In the present work, a straightforward protocol is presented with two main purposes: 1) to enhance sensitivity of the fluorogenic approach addressing caspase 3/7 activity in tissues showing scarce enzyme concentration such as skeletal muscle, and 2) to reduce/economize the volume of employed reagents. The enzyme extraction procedure, peptide substrate, dithiothreitol concentration and detection settings were appropriately optimized for use in microtiter-plate fluorometers. As a result, low to high enzyme activity extracts (from 10,000 to 260,000 relative fluorescence units) can be measured under developed sampling and experimental conditions. The fact that enzyme reactions took place in 96-microtiter well plates reduces the consumption of chemical compounds when analysing a high number of samples, thus contributing to environment sustainability.

Keywords

Caspase 3/7 activity Ac-DEVD-AMC peptide substrate apoptosis method development meat extracts rapid assays

Get full access to this article

View all access options for this article.

References

Cao

Zou

Zhang

Khan

, et al. (2013). Activation of caspase-3 and its correlation with shear force in bovine skeletal muscles during postmortem conditioning. Journal of Animal Science 91(9): 4547–4552.

Chakrabarty

Hazra

Chakraborty

Sarkar

(2004). Dynamics of solvation and rotational relaxation in neutral Brij 35 and Brij 58 micelles. Chemical Physics Letters 392(4–6): 340–347.

Chen

Feng

Zhou

, et al. (2011). Effects of camptothecin, etoposide and Ca2+ on caspase-3 activity and myofibrillar disruption of chicken during postmortem ageing. Meat Science 87(3): 165–174.

Chen

Feng

Zhang

Liu

Zhang

, et al. (2015). Effects of ultrasonic processing on caspase-3, calpain expression and myofibrillar structure of chicken during Post-Mortem ageing. Food Chemistry 177: 280–287.

Grilo

Mantalaris

(2019). Apoptosis: A mammalian cell bioprocessing perspective. Biotechnology Advances 37(3): 459–475.

Gurtu

Kain

Zhang

(1997). Fluorometric and colorimetric detection of caspase activity associated with apoptosis. Analytical Biochemistry 251(1): 98–102.

Huang

Zhang

Guo

Zhang

Zhou

(2014). Cleavage of the calpain inhibitor, calpastatin, during postmortem ageing of beef skeletal muscle. Food Chemistry 148: 1–6.

Ishisaka

Utsumi

Yabuki

Kanno

Furuno

Inoue

, et al. (1998). Activation of caspase-3-like protease by digitonin-treated lysosomes. FEBS Letters 435(2–3): 233–236.

Jia

Hildrum

Westad

Kummen

Aass

Hollung

(2006). Changes in enzymes associated with energy metabolism during the early post mortem period in longissimus thoracis bovine muscle analyzed by proteomics. Journal of Proteome Research 5(7): 1763–1769.

10.

Kemp

King

Shackelford

Wheeler

Koohmaraie

(2009). The caspase proteolytic system in callipyge and normal lambs in longissimus, semimembranosus, and infraspinatus muscles during postmortem storage. Journal of Animal Science 87(9): 2943–2951.

11.

Kemp

Bardsley

Parr

(2006a). Changes in caspase activity during the postmortem conditioning period and its relationship to shear force in porcine longissimus muscle. Journal of Animal Science 84(10): 2841–2846.

12.

Kemp

Parr

Bardsley

Buttery

PJ.

(2006b). Comparison of the relative expression of caspase isoforms in different porcine skeletal muscles. Meat Science 73(3): 426–431.

13.

Lin

Guidotti

(2009). Purification of membrane proteins. In: Methods in Enzymology. Vol. 463. Cambridge, MA: Academic Press, pp.619–629.

14.

McIlwain

Berger

Mak

TW.

(2013). Caspase functions in cell death and disease. Cold Spring Harbor Perspectives in Biology 5(4): a008656.

15.

Melody

Lonergan

Rowe

Huiatt

Mayes

Huff-Lonergan

(2004). Early postmortem biochemical factors influence tenderness and water-holding capacity of three porcine muscles. Journal of Animal Science 82(4): 1195–1205.

16.

Ouali

Herrera-Mendez

Coulis

Becila

Boudjellal

Aubry

, et al. (2006). Revisiting the conversion of muscle into meat and the underlying mechanisms. Meat Science 74(1): 44–58.

17.

Stennicke

Salvesen

GS.

(1997). Biochemical characteristics of caspases-3, -6, -7, and -8. The Journal of Biological Chemistry 272(41): 25719–25723.

18.

Stennicke

Salvesen

GS.

(1999). Caspases: preparation and characterization. Methods (San Diego, Calif.) 17(4): 313–319.

19.

Taylor

Cullen

Martin

SJ.

(2008). Apoptosis: controlled demolition at the cellular level. Nature Reviews. Molecular Cell Biology 9(3): 231–241.

20.

Wang

Liao

Diwu

(2005). N-DEVD-N′-morpholinecarbonyl-rhodamine 110: novel caspase-3 fluorogenic substrates for cell-based apoptosis assay. Bioorganic & Medicinal Chemistry Letters 15(9): 2335–2338.

21.

Zhang

Han

Chen

Han

(2017). Study on the apoptosis mediated by cytochrome c and factors that affect the activation of bovine longissimus muscle during postmortem aging. Apoptosis: An International Journal on Programmed Cell Death 22(6): 777–785.

22.

Zhang

Pan

Cao

(2013). Changes in the major caspases involved in cytoskeletal degradation of goose muscle during prolonged aging. Food Research International 51(2): 603–610.

Supplementary Material

Please find the following supplemental material available below.

For Open Access articles published under a Creative Commons License, all supplemental material carries the same license as the article it is associated with.

For non-Open Access articles published, all supplemental material carries a non-exclusive license, and permission requests for re-use of supplemental material or any part of supplemental material shall be sent directly to the copyright owner as specified in the copyright notice associated with the article.

0.00 MB

0.04 MB

Optimization of a fluorogenic assay to determine caspase 3/7 activity in meat extracts

Abstract

Keywords

Get full access to this article

References

Supplementary Material