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猪肝sn-1,2-二酰基甘油胆碱磷酸转移酶:部分纯化酶的混合胶束测定及动力学分析

sn-1,2-diacylglycerol cholinephosphotransferase from pig liver: mixed micellar assay and kinetic analysis of the partially pure enzyme.

作者信息

Bru R, Blöchliger E, Luisi P L

机构信息

Institut für Polymere, ETH-Zentrum, Zürich, Switzerland.

出版信息

Arch Biochem Biophys. 1993 Dec;307(2):295-303. doi: 10.1006/abbi.1993.1592.

DOI:10.1006/abbi.1993.1592
PMID:8274015
Abstract

sn-1,2-Diacylglycerol cholinephosphotransferase from pig liver microsomes was partially purified through a procedure involving solubilization with sodium cholate and chromatography on Sepharose 6B. The resulting preparation was 19-fold enriched with respect to microsomes and was shown to be very sensitive to different detergents. Sodium cholate gave the best yields in activity. In a mixed micellar assay with Triton X-100 a strong dependence of the enzyme activity on the concentration of mixed micelles was observed, due to Triton X-100 acting as an inactivator. Soja phosphatidylcholine added exogenously protected the enzyme against detergent inactivation and stimulated the enzyme activity. Dioleoyl-phosphatidylcholine had a similar stimulatory effect, whereas didecanoyl- or dioctanoyl-phosphatidylcholine did not; thus long-chain phosphatidylcholines seem to be essential in the activation of cholinephosphotransferase. In a mixed micellar assay with sodium cholate no inactivation of the enzyme could be detected and it was found that soja phosphatidylcholine stimulates the activity in a greater extent than in Triton X-100 mixed micelles. The phospholipid activates the enzyme in a noncompetitive way with an activation constant of 176 mol%. Km was estimated as 1.54 mol% with a Vmax = 30 nmol/min/mg protein. Those results support an activation mechanism by phosphatidylcholine interacting at sites different from the active center. The high activation constant led to the conclusion that cholinephosphotransferase requires a lipidic boundary for full activation. No activation by substrate was observed. Short-chain diacylglycerides such as dihexanoyl-, dioctanoyl-, or didecanoylglycerol can be used as substrates although the enzyme in this case has only 5 to 10% of the activity it has for dioleoylglycerol or egg diglycerides.

摘要

猪肝微粒体中的sn-1,2-二酰基甘油胆碱磷酸转移酶通过用胆酸钠增溶和在琼脂糖凝胶6B上进行色谱分离的方法进行了部分纯化。所得制剂相对于微粒体富集了19倍,并且显示出对不同去污剂非常敏感。胆酸钠的活性产率最高。在与 Triton X-100的混合胶束测定中,观察到酶活性强烈依赖于混合胶束的浓度[,这是因为Triton X-100起到了失活剂的作用]。外源添加的大豆磷脂酰胆碱可保护该酶免受去污剂失活并刺激酶活性。二油酰磷脂酰胆碱具有类似的刺激作用,而二癸酰或二辛酰磷脂酰胆碱则没有;因此,长链磷脂酰胆碱似乎是胆碱磷酸转移酶激活所必需的。在与胆酸钠的混合胶束测定中,未检测到酶的失活,并且发现大豆磷脂酰胆碱比在Triton X-100混合胶束中更能刺激活性。磷脂以非竞争性方式激活该酶,激活常数为176 mol%。Km估计为1.54 mol%,Vmax = 30 nmol/分钟/毫克蛋白质。这些结果支持磷脂酰胆碱在不同于活性中心的位点相互作用的激活机制。高激活常数得出结论,胆碱磷酸转移酶需要脂质边界才能完全激活。未观察到底物的激活作用。短链二酰基甘油,如二己酰、二辛酰或二癸酰甘油,可以用作底物,尽管在这种情况下该酶的活性仅为其二油酰甘油或蛋黄甘油二酯活性的5%至10%。 (方括号内为补充完整语义的内容)

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引用本文的文献

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