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宰后贮藏期间,美臀羊和正常羔羊背最长肌、半膜肌和冈下肌中的半胱天冬酶蛋白水解系统。

The caspase proteolytic system in callipyge and normal lambs in longissimus, semimembranosus, and infraspinatus muscles during postmortem storage.

作者信息

Kemp C M, King D A, Shackelford S D, Wheeler T L, Koohmaraie M

机构信息

Roman L. Hruska US Meat Animal Research Center, USDA, ARS, Clay Center, NE 68933-0166, USA.

出版信息

J Anim Sci. 2009 Sep;87(9):2943-51. doi: 10.2527/jas.2009-1790. Epub 2009 May 6.

Abstract

The objective of this experiment was to determine whether the caspase proteolytic system has a role in postmortem tenderization. Six ewes and 6 wethers that were noncarriers and 6 ewes and 6 wethers that were expressing the callipyge gene were used for this study. Caspase activities were determined in LM at 7 different time points during the postmortem storage period: 0 h, 4 h, 8 h, 24 h, 2 d, 7 d, and 21 d and in semimembranosus (SM) and infraspinatus (IS) muscles at 0 h, 8 h, 24 h, and 7 d from callipyge and noncallipyge (normal) lambs. Calpastatin activity was determined at 0 h, 2 d, 7 d, and 21 d and slice shear force measured at 2, 7, and 21 d in the LM. Calpastatin activity and slice shear force were greater in LM from callipyge lambs than normal lambs at each time point (P < 0.001 and P < 0.0001, respectively). Caspases 3 and 7 are executioner caspases, and their combined activity was found to decrease during the postmortem storage period in LM, SM, and IS muscles from callipyge and normal lambs. Similarly, activity of the initiator caspase (caspase 9) decreased (P < 0.05) in all 3 muscles across the postmortem storage period in callipyge and normal lambs, and its decrease in activity preceded that of the executioner caspases 3/7. A positive relationship also was detected between caspase 9 and caspase 3/7 in LM, SM, and IS muscles (P < 0.0001, r = 0.85, r = 0.86, r = 0.84, respectively), which is consistent with caspase 9 being responsible for the cleavage and activation of the executioner caspases (caspase 3/7) downstream. Caspase 3/7 and caspase 9 activities at 8 h in SM were greater in normal lamb than callipyge lamb (P < 0.05), with a trend for caspase 3/7 activity to be greater at 24 h postmortem (P = 0.0841). There also was a trend for caspase 3/7 activity to be greater in LM at 21 d in normal lamb than in callipyge lamb (P = 0.053), although there were no differences detected in caspase activities between genotypes in the IS muscle, which is not affected by the callipyge gene. A negative relationship also was detected between peak caspase 3/7 activity at 8 h in LM from normal lambs and calpastatin activity at 0 and 2 d (r = -0.65, r = -0.68, respectively, P < 0.05). This relationship was not observed in LM from callipyge lambs, suggesting that caspase 3/7 may be cleaving calpastatin in normal lambs but the level of calpastatin in callipyge lambs is such that caspase 3/7 cannot degrade it sufficiently to overcome the increased content of calpastatin, and thus, calpastatin activity is the overriding factor in postmortem proteolysis in these animals. There was no direct evidence from this study that caspases have a significant role in postmortem tenderization, but they may have some role through calpastatin degradation.

摘要

本实验的目的是确定半胱天冬酶蛋白水解系统在宰后嫩化过程中是否起作用。本研究使用了6只非携带型母羊和6只非携带型阉羊,以及6只表达臀肌肥大基因的母羊和6只表达臀肌肥大基因的阉羊。在宰后储存期的7个不同时间点(0小时、4小时、8小时、24小时、2天、7天和21天)测定腰大肌(LM)中的半胱天冬酶活性,并在宰后0小时、8小时、24小时和7天测定来自臀肌肥大和非臀肌肥大(正常)羔羊的半膜肌(SM)和冈下肌(IS)中的半胱天冬酶活性。在0小时、2天、7天和21天测定钙蛋白酶抑制蛋白活性,并在第2天、7天和21天测定腰大肌中的切片剪切力。在每个时间点,臀肌肥大羔羊腰大肌中的钙蛋白酶抑制蛋白活性和切片剪切力均高于正常羔羊(分别为P < 0.001和P < 0.0001)。半胱天冬酶3和7是执行性半胱天冬酶,发现在宰后储存期,臀肌肥大和正常羔羊的腰大肌、半膜肌和冈下肌中,它们的联合活性降低。同样地,在宰后储存期,启动性半胱天冬酶(半胱天冬酶9)在臀肌肥大和正常羔羊的所有3块肌肉中的活性均降低(P < 0.05),且其活性降低先于执行性半胱天冬酶3/7。在腰大肌、半膜肌和冈下肌中还检测到半胱天冬酶9与半胱天冬酶3/7之间存在正相关关系(分别为P < 0.0001,r = 0.85、r = 0.86、r = 0.84),这与半胱天冬酶9负责下游执行性半胱天冬酶(半胱天冬酶3/7)的切割和激活一致。正常羔羊半膜肌在8小时时的半胱天冬酶3/7和半胱天冬酶9活性高于臀肌肥大羔羊(P < 0.05),宰后24小时时半胱天冬酶3/7活性有升高趋势(P = 0.0841)。正常羔羊腰大肌在21天时的半胱天冬酶3/7活性也有高于臀肌肥大羔羊的趋势(P = 0.053),尽管在不受臀肌肥大基因影响的冈下肌中未检测到基因型间半胱天冬酶活性的差异。在正常羔羊腰大肌8小时时的半胱天冬酶3/7峰值活性与0天和2天时的钙蛋白酶抑制蛋白活性之间也检测到负相关关系(分别为r = -0.65、r = -0.68,P < 0.05)。在臀肌肥大羔羊的腰大肌中未观察到这种关系,这表明半胱天冬酶3/7可能在正常羔羊中切割钙蛋白酶抑制蛋白,但臀肌肥大羔羊中的钙蛋白酶抑制蛋白水平使得半胱天冬酶3/7无法充分降解它以克服钙蛋白酶抑制蛋白含量的增加,因此,钙蛋白酶抑制蛋白活性是这些动物宰后蛋白水解的主要因素。本研究没有直接证据表明半胱天冬酶在宰后嫩化中起重要作用,但它们可能通过钙蛋白酶抑制蛋白降解发挥一定作用。

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