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中链脂肪酰辅酶A合成酶的研究。纯化及性质

Studies on medium-chain fatty acyl-coenzyme a synthetase. Purification and properties.

作者信息

Bar-Tana J, Rose G, Shapiro B

出版信息

Biochem J. 1968 Sep;109(2):269-74. doi: 10.1042/bj1090269.

Abstract
  1. Medium-chain fatty acyl-CoA synthetase (EC 6.2.1.2) was isolated by the method of Mahler, Wakil & Bock (1953) and the enzyme activity determined by the disappearance of CoA in the presence either of butyrate and ATP or of butyryl-AMP, as well as by ATP formation from butyryl-AMP and PP(i). 2. Preincubation of the enzyme with CoA and ATP alone or together, followed by the removal of these substrates by gel filtration, caused a marked inhibition of ATP formation, contrary to results previously obtained with palmitoyl-CoA synthetase. 3. The effect of ATP on butyryl-AMP-dependent CoA disappearance was inconsistent. Low concentrations of ATP (0.1-0.5mm) always caused inhibition, whereas higher concentrations (5-10mm) activated in some enzyme preparations and inhibited in others. 4. This inconsistency was shown to be due to the presence of two enzyme fractions. Both fractions had similar activities when assayed by the butyryl-AMP- or butyrate-plus-ATP-dependent CoA disappearance. However, fraction I was activated by ATP as measured by butyryl-AMP-dependent CoA disappearance whereas fraction II was inhibited by it. Fraction I also catalysed ATP formation from butyryl-AMP and PP(i) whereas fraction II was lacking in such activity. 5. The relationship of these observations with respect to other known mechanisms of fatty acid-activating systems is discussed.
摘要
  1. 中链脂肪酰辅酶A合成酶(EC 6.2.1.2)采用马勒、瓦基尔和博克(1953年)的方法进行分离,通过在丁酸盐和ATP存在下或丁酰-AMP存在下辅酶A的消失,以及由丁酰-AMP和焦磷酸(PP(i))形成ATP来测定酶活性。2. 将酶单独或与辅酶A和ATP一起预孵育,随后通过凝胶过滤去除这些底物,导致ATP形成受到显著抑制,这与先前用棕榈酰辅酶A合成酶获得的结果相反。3. ATP对丁酰-AMP依赖性辅酶A消失的影响并不一致。低浓度的ATP(0.1 - 0.5mmol/L)总是导致抑制,而较高浓度(5 - 10mmol/L)在一些酶制剂中起激活作用,在另一些中则起抑制作用。4. 这种不一致被证明是由于存在两种酶组分。当通过丁酰-AMP或丁酸盐加ATP依赖性辅酶A消失进行测定时,两种组分具有相似的活性。然而,以丁酰-AMP依赖性辅酶A消失来衡量,组分I被ATP激活,而组分II被其抑制。组分I还催化由丁酰-AMP和PP(i)形成ATP,而组分II缺乏这种活性。5. 讨论了这些观察结果与脂肪酸激活系统其他已知机制的关系。

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