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在钠钾ATP酶中,伴随寡霉素诱导的钠离子结合形式的形成及其向ADP敏感型磷酸酶的转化而发生的构象变化。

Conformational change accompanying formation of oligomycin-induced Na(+)-bound forms and their conversion to ADP-sensitive phosphoenzymes in Na+,K(+)-ATPase.

作者信息

Taniguchi K, Sasaki T, Shinoguchi E, Kamo Y, Ito E

机构信息

Department of Chemistry, Faculty of Science, Hokkaido University.

出版信息

J Biochem. 1991 Feb;109(2):299-306.

PMID:1650775
Abstract

Oligomycin reduced the fluorescence intensity of an N-(p-(2-benzimidazoly)phenyl) maleimide (BIPM) probe at Cys-964 of the alpha-chain of pig kidney Na+,K(+)-ATPase with increase in the concentration of Na+ with a Hill coefficient of nh = 0.77 with Kh = 231 mM. The maximum fluorescence decrease was around 80% of the value observed after accumulation of ADP-sensitive phosphoenzyme (E1P) in the presence of 2 M Na+. The addition of Mg2+ and ATP with Na+ or choline chloride to give the same final ligand concentration to the Na(+)-enzyme-oligomycin complex formed with 16 mM Na+ + 1,984 mM choline chloride or 2 M Na+ induced rapid phosphorylation (20 or 21/s) and slower fluorescence decrease (12.1 +/- 1.2 or 10.1 +/- 3.2/s). These additions to the Na(+)-enzyme complex formed under the former or the latter conditions induced slow phosphorylation (13/s) prior to a much slower fluorescence decrease (3.4 +/- 0.3 or 8.6 +/- 0.7/s). The addition of Ca2+ and ATP to these enzyme complexes induced rapid fluorescence changes (21-11/s) followed by one order of magnitude slower rates of phosphorylation (1.5-1.3 s). These data suggest that the decrease in BIPM fluorescence induced by ATP with Ca2+ or with Mg2+, reflects the change of the Na+ binding state before or after the formation of E1P, respectively.

摘要

寡霉素降低了猪肾Na⁺,K⁺-ATP酶α链Cys-964位点处N-(对-(2-苯并咪唑基)苯基)马来酰亚胺(BIPM)探针的荧光强度,随着Na⁺浓度增加,希尔系数nh = 0.77,Kh = 231 mM。最大荧光下降约为在2 M Na⁺存在下积累ADP敏感磷酸酶(E1P)后观察到的值的80%。向与16 mM Na⁺ + 1,984 mM氯化胆碱或2 M Na⁺形成的Na⁺-酶-寡霉素复合物中添加Mg²⁺和ATP或氯化胆碱以达到相同的最终配体浓度,诱导快速磷酸化(20或21/s)和较慢的荧光下降(12.1±1.2或10.1±3.2/s)。在前者或后者条件下形成的Na⁺-酶复合物中添加这些物质,在荧光下降慢得多(3.4±0.3或8.6±0.7/s)之前诱导缓慢磷酸化(13/s)。向这些酶复合物中添加Ca²⁺和ATP诱导快速荧光变化(21 - 11/s),随后磷酸化速率慢一个数量级(1.5 - 1.3/s)。这些数据表明,ATP与Ca²⁺或与Mg²⁺诱导的BIPM荧光下降分别反映了E1P形成之前或之后Na⁺结合状态的变化。

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