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非离子去污剂对心肌微粒体和肌膜腺苷酸环化酶的不同作用

Differential effects of non-ionic detergents on microsomal and sarcolemmal adenylate cyclase in cardiac muscle.

作者信息

Sulakhe P V, Narayanan N

出版信息

Biochem J. 1978 Oct 1;175(1):171-80. doi: 10.1042/bj1750171.

Abstract
  1. About 4 and 23% of the homogenate adenylate cyclase activity was recovered in the microsomal and sarcolemmal fractions isolated from guinea-pig heart ventricles. 2. Cardiac microsomal adenylate cyclase activity [basal as well as p[NH]ppG (guanyl-5'-yl imidodiphosphate)- and NaF-stimulated] was increased over 2-fold in the presence of Lubrol-PX (0.01-0.1%). 3. The sarcolemmal enzyme, however, showed concentration-dependent inhibition caused by the detergent under all assay conditions, except when p[NH]ppG was included in the assay. In the latter case, the detergent (0.01-0.02%) caused a modest increase (30-45%) in enzyme activity. 4. Another non-ionic detergent, Triton X-100, also stimulated the microsomal cyclase and inhibited the sarcolemmal enzyme. 5. With either membrane fraction, Lubrol-PX solubilized the enzyme when the detergent/membrane protein ratio was 2.5 (mumol of detergent/mg of protein). 6. The findings with homogenate and a washed particulate fraction resembled those obtained with sarcolemma, and those with isolated sarcoplasmic reticulum resembled those with microsomal preparations. 7. p[NH]ppG, and to some extent NaF, protected the detergent-induced inactivation of the enzyme observed at higher detergent concentrations (0.5% Lubrol-PX and 0.05-0.5% Triton X-100). 8. In the absence of detergents, p[NH]ppG increased the basal enzyme activity about 2-fold in microsomal fractions, but did not appreciably stimulate the sarcolemmal enzyme. Isoproterenol, on the other hand, increased the sarcolemmal enzyme activity (>2-fold) in the presence of p[NH]ppG and caused only moderate stimulation (31%) of the microsomal enzyme under these conditions. 9. These findings support the view that, although the bulk of adenylate cyclase resides in heart sarcolemma (plasma membrane), the microsomal activity cannot be accounted for solely by contamination of the microsomal fraction with sarcolemma, as has been suggested by others [Besch, Jones & Watanabe (1976) Circ. Res.39, 586-595; Engelhard, Plut & Storm (1976) Biochim. Biophys. Acta451, 48-61]. Further, the results of this study show that cardiac sarcoplasmic-reticulum membranes possess this enzyme.
摘要
  1. 从豚鼠心室分离得到的微粒体和肌膜组分中,分别回收了约4%和23%的匀浆腺苷酸环化酶活性。2. 在存在Lubrol-PX(0.01 - 0.1%)的情况下,心脏微粒体腺苷酸环化酶活性(基础活性以及对[NH]ppG(鸟苷-5'-亚氨二磷酸)和NaF刺激的活性)增加了2倍以上。3. 然而,在所有测定条件下,除了测定中包含[NH]ppG时,去污剂对肌膜酶表现出浓度依赖性抑制。在后一种情况下,去污剂(0.01 - 0.02%)使酶活性适度增加(30 - 45%)。4. 另一种非离子去污剂Triton X-100也刺激微粒体环化酶并抑制肌膜酶。5. 对于任何一种膜组分,当去污剂/膜蛋白比例为2.5(去污剂微摩尔数/蛋白毫克数)时,Lubrol-PX可溶解该酶。6. 匀浆和洗涤后的颗粒组分的结果与肌膜的结果相似,而分离的肌浆网的结果与微粒体制剂的结果相似。7. [NH]ppG以及在一定程度上NaF可保护在较高去污剂浓度(0.5% Lubrol-PX和0.05 - 0.5% Triton X-100)下观察到的去污剂诱导的酶失活。8. 在没有去污剂的情况下,[NH]ppG使微粒体组分中的基础酶活性增加约2倍,但对肌膜酶没有明显刺激。另一方面,在存在[NH]ppG的情况下,异丙肾上腺素增加了肌膜酶活性(>2倍),并且在这些条件下仅对微粒体酶产生适度刺激(31%)。9. 这些发现支持这样一种观点,即尽管大部分腺苷酸环化酶存在于心脏肌膜(质膜)中,但微粒体活性不能仅由微粒体组分被肌膜污染来解释,正如其他人所提出的那样[Besch,Jones和Watanabe(1976年)《循环研究》39,586 - 595;Engelhard,Plut和Storm(1976年)《生物化学与生物物理学报》451,48 - 61]。此外,本研究结果表明心脏肌浆网膜具有这种酶。

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