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短期禁食对肝脏微粒体谷胱甘肽-胰岛素转氢酶的影响。

Effect of a short-term fast on hepatic microsomal glutathione-insulin transhydrogenase.

作者信息

Striffler J S

出版信息

Diabete Metab. 1985 Dec;11(6):368-75.

PMID:4085684
Abstract

The effect of nutritional state on the hepatic insulin degrading enzyme glutathione-insulin transhydrogenase (GIT) was assessed by comparing the distribution of GIT activity between its nonlatent and latent forms in fractionated liver microsomes from ad lib fed (n = 11) and overnight fasted (n = 11) rats. In fed state microsomes, treatment with the membrane disrupting agent phospholipase-A2 (PLA2) over a range of PLA2 concentrations (less than or equal to 2.0 micrograms/ml) caused biphasic release of GIT with a peak activity of 651 +/- 58 U/mg microsomal protein (n = 11) occurring at PLA2 = 1.0 microgram/ml. In total liver microsomes from fasted animals, GIT release in response to PLA2 was sigmoidal over the entire range of PLA2 concentrations, with a plateau of activities (450 U/mg microsomal protein) occurring at PLA2 greater than or equal to 0.75 microgram/ml. Peak activities (478 +/- 88 U/mg prot., n = 11, PLA2 = 1.0 microgram/ml) were 30% lower as compared to the fed state (p less than .05). In untreated (intact) microsomes from fed rat liver nonlatent activity was 126 +/- 8 U/mg protein, representing 19.9 +/- 1.2% of the total GIT activity. In contrast, nonlatent activity measurable in suspensions of intact microsomes from fasted rat liver (110 +/- 6 U/mg) expressed as a % of total activity was significantly increased (p less than .05) being 23.3 +/- 1.1%. Similar fasting-induced changes were also apparent in isolated smooth microsomes but not in rough membrane preparations.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过比较自由进食(n = 11)和禁食过夜(n = 11)大鼠分级肝微粒体中谷胱甘肽 - 胰岛素转氢酶(GIT,一种肝胰岛素降解酶)非潜伏形式和潜伏形式之间的活性分布,评估营养状态对其的影响。在进食状态的微粒体中,用膜破坏剂磷脂酶 - A2(PLA2)在一系列PLA2浓度(小于或等于2.0微克/毫升)下处理,导致GIT呈双相释放,在PLA2 = 1.0微克/毫升时出现峰值活性651±58 U/毫克微粒体蛋白(n = 11)。在禁食动物的全肝微粒体中,响应PLA2的GIT释放在整个PLA2浓度范围内呈S形,在PLA2大于或等于0.75微克/毫升时出现活性平台(450 U/毫克微粒体蛋白)。峰值活性(478±88 U/毫克蛋白,n = 11,PLA2 = 1.0微克/毫升)比进食状态低30%(p <.05)。在来自进食大鼠肝脏的未处理(完整)微粒体中,非潜伏活性为126±8 U/毫克蛋白,占总GIT活性的19.9±1.2%。相比之下,在来自禁食大鼠肝脏的完整微粒体悬浮液中可测量的非潜伏活性(110±6 U/毫克)占总活性的百分比显著增加(p <.05),为23.3±1.1%。类似的禁食诱导变化在分离的平滑微粒体中也很明显,但在粗糙膜制剂中不明显。(摘要截断于250字)

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