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心肌肌膜的蛋白质分析:膜扰动剂对膜蛋白和钙转运的影响。

Protein analysis of cardiac sarcolemma: effects of membrane-perturbing agents on membrane proteins and calcium transport.

作者信息

St Louis P J, Sulakhe P V

出版信息

Biochemistry. 1978 Oct 17;17(21):4540-50. doi: 10.1021/bi00614a028.

Abstract

Protein composition of cardiac sarcolemmal membranes was analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Membranes were observed to contain about 20 polypeptide bands ranging from 18000 to 200 000 dalton mass. Out of these, six bands were prominent and together comprised 57% of the membrane protein. When sarcolemmal membranes, phosphorylated by [gamma-(32)P] ATP in the presence of Ca(2+) or Na+ with and without K+, were fractionated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis at pH 2.4, the band III region (Mr 105 000) of gels was found to contain active sites of monomeric Ca-ATPase and (Na,K)ATPase. Bands I (Mr greater than 200 000), II (Mr 150 000), III (Mr 105 000), and VI (Mr 47 000) were accesible to trypsin; the extent of proteolysis was dependent on the time of exposure to, and the concentration of, trypsin (i.e, ratio of sarcolemmal protein/trypsin). Addition of molar sucrose protected sarcolemmal proteins from the tryptic proteolysis. Calcium transport was reduced by the action of trypsin; the degree of reduction was influenced by the time of exposure of membranes to trypsin as well as the concentration of trypsin. (Mg,Ca)ATPase activity, on the other hand, was elevated moderately at lower concentration and reduced at higher concentration of trypsin. Treatment with phospholipase C cium transport and (Mg,Ca)ATPase activity; electrophoretic patterns were unaffected by this treatment. Addition of lecithin to phospholipase C treated membranes produced a moderate increase in calcium transport. Exposure to Triton X-100 (1%) specifically solubilized three protein bands (Mr90 000, 67 000, and 57 000), whereas exposure to deoxycholate (1%) preferentially solubilized high-molecular-weight proteins, including band III (Mr 105 000); Lubrol-PX (1%) caused nonspecific solubilization of proteins, although the extent of solubilization with Lubrol-PX was considerably less than with either Triton or deoxycholate.

摘要

采用十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳分析心肌肌膜的蛋白质组成。观察到膜中含有约20条多肽带,分子量范围从18000到200000道尔顿。其中,6条带显著,共占膜蛋白的57%。当肌膜在有或无K⁺存在的情况下,于Ca²⁺或Na⁺存在时被[γ-(³²)P]ATP磷酸化,然后在pH 2.4条件下通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳进行分级分离时,发现凝胶的带III区域(Mr 105000)含有单体Ca - ATP酶和(Na,K)ATP酶的活性位点。带I(Mr大于200000)、带II(Mr 150000)、带III(Mr 105000)和带VI(Mr 47000)可被胰蛋白酶作用;蛋白水解程度取决于胰蛋白酶的作用时间和浓度(即肌膜蛋白/胰蛋白酶的比例)。添加摩尔蔗糖可保护肌膜蛋白免受胰蛋白酶水解。胰蛋白酶的作用会降低钙转运;降低程度受膜与胰蛋白酶作用时间以及胰蛋白酶浓度的影响。另一方面,(Mg,Ca)ATP酶活性在胰蛋白酶浓度较低时适度升高,在较高浓度时降低。用磷脂酶C处理会影响钙转运和(Mg,Ca)ATP酶活性;电泳图谱不受此处理影响。向经磷脂酶C处理的膜中添加卵磷脂会使钙转运适度增加。暴露于Triton X - 100(1%)会特异性溶解三条蛋白带(Mr 90000、67000和57000),而暴露于脱氧胆酸盐(1%)会优先溶解高分子量蛋白,包括带III(Mr 105000);Lubrol - PX(1%)会导致蛋白非特异性溶解,尽管Lubrol - PX的溶解程度远低于Triton或脱氧胆酸盐。

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