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AMP对肌肉特异性AMP激活蛋白激酶α2β2γ3复合物的调节以及γ3亚基突变对该酶AMP依赖性的影响。

Regulation of the muscle-specific AMP-activated protein kinase alpha2beta2gamma3 complexes by AMP and implications of the mutations in the gamma3-subunit for the AMP dependence of the enzyme.

作者信息

Lindgren Kerstin, Ormestad Mattias, Persson Mårten, Martinsson Sofia, Svensson L Thomas, Mahlapuu Margit

机构信息

Discovery Research, Biovitrum AB, Biotech Center, Arvid Wallgrens Backe 20, SE-413 46 Göteborg, Sweden.

出版信息

FEBS J. 2007 Jun;274(11):2887-96. doi: 10.1111/j.1742-4658.2007.05821.x.

DOI:10.1111/j.1742-4658.2007.05821.x
PMID:17518971
Abstract

The AMP-activated protein kinase is an evolutionarily conserved heterotrimer that is important for metabolic sensing in all eukaryotes. The muscle-specific isoform of the regulatory gamma-subunit of the kinase, AMP-activated protein kinase gamma3, has a key role in glucose and fat metabolism in skeletal muscle, as suggested by metabolic characterization of humans, pigs and mice harboring substitutions in the AMP-binding Bateman domains of gamma3. We demonstrate that AMP-activated protein kinase alpha2beta2gamma3 trimers are allosterically activated approximately three-fold by AMP with a half-maximal stimulation (A(0.5)) at 1.9 +/- 0.5 or 2.6 +/- 0.3 microm, as measured for complexes expressed in Escherichia coli or mammalian cells, respectively. We show that mutations in the N-terminal Bateman domain of gamma3 (R225Q, H306R and R307G) increased the A(0.5) values for AMP, whereas the fold activation of the enzyme by 200 microm AMP remained unchanged in comparison to the wild-type complex. The mutations in the C-terminal Bateman domain of gamma3 (H453R and R454G), on the other hand, substantially reduced the fold stimulation of the complex by 200 microm AMP, and resulted in AMP dependence curves similar to those of the double mutant, R225Q/R454G. A V224I mutation in gamma3, known to result in a reduced glycogen content in pigs, did not affect the fold activation or the A(0.5) values for AMP. Importantly, we did not detect any increase in phosphorylation of Thr172 of alpha2 by the upstream kinases in the presence of increasing concentrations of AMP. Taken together, the data show that different mutations in gamma3 exert different effects on the allosteric regulation of the alpha2beta2gamma3 complex by AMP, whereas we find no evidence for their role in regulating the level of phosphorylation of alpha2 by upstream kinases.

摘要

AMP 激活的蛋白激酶是一种进化上保守的异源三聚体,对所有真核生物的代谢感知都很重要。激酶调节性γ亚基的肌肉特异性同工型,即 AMP 激活的蛋白激酶γ3,在骨骼肌的葡萄糖和脂肪代谢中起关键作用,这一点已通过对γ3 的 AMP 结合贝特曼结构域中存在替代突变的人类、猪和小鼠的代谢特征分析得到证实。我们证明,AMP 激活的蛋白激酶α2β2γ3 三聚体被 AMP 变构激活约三倍,在大肠杆菌或哺乳动物细胞中表达的复合物中,半最大刺激浓度(A(0.5))分别为 1.9±0.5 或 2.6±0.3 微摩尔。我们发现,γ3 的 N 端贝特曼结构域中的突变(R225Q、H306R 和 R307G)增加了 AMP 的 A(0.5)值,而与野生型复合物相比,200 微摩尔 AMP 对该酶的激活倍数保持不变。另一方面,γ3 的 C 端贝特曼结构域中的突变(H453R 和 R454G)显著降低了 200 微摩尔 AMP 对复合物的激活倍数,并导致 AMP 依赖性曲线与双突变体 R225Q/R454G 相似。γ3 中的 V224I 突变已知会导致猪体内糖原含量降低,但不影响 AMP 的激活倍数或 A(0.5)值。重要的是,在 AMP 浓度增加的情况下,我们未检测到上游激酶对α2 的 Thr172 磷酸化有任何增加。综上所述,数据表明γ3 中的不同突变对 AMP 对α2β2γ3 复合物的变构调节有不同影响,而我们没有发现它们在调节上游激酶对α2 的磷酸化水平方面起作用的证据。

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