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纤细裸藻中的特异性磷酸化酶可裂解5',5'''-P(1),P(4)-四磷酸二腺苷(Ap(4)A)和5',5'''-P(1),P(3)-三磷酸二腺苷(Ap(3)A)。

Specific phosphorylase from Euglena gracilis splits diadenosine 5',5'''-P(1),P(4)-tetraphosphate (Ap(4)A) and diadenosine 5',5'''-P(1),P(3)-triphosphate (Ap(3)A).

作者信息

Guranowski A, Starynska E, Wasternack C

出版信息

Int J Biochem. 1988;20(4):449-55. doi: 10.1016/0020-711x(88)90214-5.

Abstract
  1. Phosphorolytic cleavage of Ap(4),A was demonstrated in cell-free extracts from two protozoan organisms, Euglena gracilis and Acanthamoeba castellanii. 2. A specific dinucleoside oligophosphate (DNOP) alpha, beta-phosphorylase which degrades substrates with formation of corresponding nucleoside 5'-diphosphate (NDP) as one of the reaction products was purified 625-fold from Euglena gracilis cells. 3. In addition to Ap(4)A, the phosphorylase degrades AP(3)A, Ap(5)A, Gp(4)G and one of phosphonate analogs, ApppCH(2)pA. The K(m) values for Ap(4), A and Ap(3) A are 27 and 25 micron, and relative velocities 100 and 14, respectively. The K(m) for phosphate is 0.5 mM. 4. Some anions (arsenate, chromate, molybdate and vanadate) can substitute for phosphate in the catalyzed reactions and in their presence the DNOPs yield corresponding nucleoside 5'-monophosphate as one of the reactions' product. The enzyme supports also an anion-dependent dephosphorylation of NDPs. 5. Molecular weight of the native Euglena phosphorylase is 30,000. Optimum pH for its activity is at 8.0 Divalent metal cations are essential for the phosphorolysis of DNOPs but are not for the NDP dephosphorylation mentioned.
摘要
  1. 在两种原生动物——纤细裸藻和卡氏棘阿米巴的无细胞提取物中证实了Ap(4)A的磷酸解裂解。2. 从纤细裸藻细胞中纯化出一种特异性二核苷寡磷酸(DNOP)α,β-磷酸化酶,该酶降解底物时会形成相应的核苷5'-二磷酸(NDP)作为反应产物之一,纯化倍数达625倍。3. 除Ap(4)A外,该磷酸化酶还能降解AP(3)A、Ap(5)A、Gp(4)G以及一种膦酸类似物ApppCH(2)pA。Ap(4)A和Ap(3)A的K(m)值分别为27和25微摩尔,相对速度分别为100和14。磷酸盐的K(m)值为0.5毫摩尔。4. 一些阴离子(砷酸盐、铬酸盐、钼酸盐和钒酸盐)可在催化反应中替代磷酸盐,在它们存在的情况下,DNOPs会产生相应的核苷5'-单磷酸作为反应产物之一。该酶还支持NDPs的阴离子依赖性去磷酸化反应。5. 天然纤细裸藻磷酸化酶的分子量为30,000。其活性的最适pH值为8.0。二价金属阳离子对于DNOPs的磷酸解是必需的,但对于上述NDP去磷酸化反应则不是必需的。

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