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Energy-dependent binding of dansylgalactoside to the lac carrier protein: direct binding measurements.

机译:丹参半乳糖苷与lac载体蛋白的能量依赖性结合:直接结合测量。

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摘要

High specific activity 6'-N-[3H]dansyl)aminohexyl 1-thio-beta-D-galactopyranoside (Dns6-Gal) has been synthesized, and its binding to Escherichia coli membrane vesicles measured directly by flow dialysis. With ML 308-225 vesicles containing the lac carrier protein, specific binding is not detected in the absence of D-lactate or reduced phenazine methosulfate. In the presence of these electron donors, binding is observed, and the binding constant and number of binding sites are approximately 4 muM and 1.5 nmol/mg of membrane protein, respectively. These values are in excellent agreement with those obtained by fluorescence titration. p-Chloromercuribenzenesulfonate, which directly inactivates the lac carrier protein, and carbonylcyanide m-chlorophenylhydrazone, which collapses the membrane potential, cause release of bound Dns6-Gal. Moreover, significant binding is not observed with membrane vesicles that are devoid of the lac carrier protein. The results provide qualitative and quantitative confirmation of previous studies which indicate that changes in dansylgalactoside fluorescence observed on "energization" of membrane vesicles reflect binding of the probe to the lac carrier protein.
机译:已经合成了高比活性的6'-N- [3H]丹酰基)氨基己基1-硫代-β-D-吡喃半乳糖苷(Dns6-Gal),其与大肠杆菌膜囊泡的结合可通过流透法直接测量。对于含有lac载体蛋白的ML 308-225囊泡,在没有D-乳酸或还原的吩嗪硫酸甲酯的情况下,未检测到特异性结合。在这些电子供体的存在下,观察到结合,结合常数和结合位点数分别为约4μM和1.5nmol / mg膜蛋白。这些值与通过荧光滴定获得的值非常一致。对氯呋喃苯磺酸盐直接使lac载体蛋白失活,而羰基氰化物间氯苯基phenyl使膜电位崩溃,导致结合的Dns6-Gal释放。而且,没有缺少lac载体蛋白的膜囊泡未观察到明显的结合。结果提供了先前研究的定性和定量证实,这些研究表明在膜囊泡“通电”时观察到的丹酰半乳糖苷荧光变化反映了探针与lac载体蛋白的结合。

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