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首页> 外文期刊>American Journal of Physiology >Characterization of RII(beta) and D-AKAP1 in differentiated adipocytes.
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Characterization of RII(beta) and D-AKAP1 in differentiated adipocytes.

机译:RIIβ和D-AKAP1在分化的脂肪细胞中的表征。

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摘要

A-kinase anchoring proteins (AKAPs) have been proposed to regulate cAMP-dependent signaling in the cell by targeting RII subunits of protein kinase A (PKA) to specific subcellular compartments. RII(beta) is the predominant PKA subtype in adipose tissue. In gel overlay assays of C3H/10T1/2 adipocytes and adipose tissue, RII(beta) bound to several proteins including a prominent 132-kDa band, which was strongly induced upon differentiation of C3H/10T1/2 cells into adipocytes. Immunoblotting and nuclease protection analysis of C3H/10T1/2 cellular extracts identified this band as D-AKAP1/S-AKAP84, a putative AKAP. Immunocytochemical analysis of C3H/10T1/2 adipocytes revealed that most of D-AKAP1/S-AKAP84, but not RII(beta), was colocalized with a mitochondrial-selective dye, MitoTracker red. These findings were further confirmed in studies where D-AKAP1/ S-AKAP84, but not RII(beta), were localized in purified mitochondria made from C3H/10T1/2 adipocytes. Moreover, D-AKAP1, which is upregulated after differentiation, did not recruit RII(beta) to membrane fractions enriched in mitochondria. These results demonstrate that D-AKAP1/S-AKAP84 does not interact with PKA in differentiated C3H/10T1/2 adipocytes under the conditions tested.
机译:已提出通过将蛋白激酶A(PKA)的RII亚基靶向特定的亚细胞区室来调节细胞中依赖cAMP的信号传导的A激酶锚定蛋白(AKAP)。 RIIβ是脂肪组织中主要的PKA亚型。在C3H / 10T1 / 2脂肪细胞和脂肪组织的凝胶覆盖测定中,RIIβ与包括突出的132-kDa条带的几种蛋白质结合,该蛋白在C3H / 10T1 / 2细胞分化为脂肪细胞时被强烈诱导。对C3H / 10T1 / 2细胞提取物的免疫印迹和核酸酶保护分析确定该条带为D-AKAP1 / S-AKAP84,一种假定的AKAP。对C3H / 10T1 / 2脂肪细胞的免疫细胞化学分析显示,大多数D-AKAP1 / S-AKAP84(而不是RIIβ)与线粒体选择性染料MitoTracker红共定位。这些发现在D-AKAP1 / S-AKAP84而非RIIβ位于由C3H / 10T1 / 2脂肪细胞制成的纯化线粒体中的研究中得到了进一步证实。此外,分化后上调的D-AKAP1不会将RIIβ募集到富集线粒体的膜部分。这些结果表明,在测试条件下,D-AKAP1 / S-AKAP84在分化的C3H / 10T1 / 2脂肪细胞中不与PKA相互作用。

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