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Dansyl-Galactoside a Fluorescent Probe of Active Transport in Bacterial Membrane Vesicles

机译:Dansyl-Galactoside细菌膜囊泡中主动转运的荧光探针

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摘要

A fluorescent galactoside, 2-(N-dansyl)-aminoethyl β-D-thiogalactoside (dansyl-galactoside), competitively inhibits lactose transport by membrane vesicles of Escherichia coli, but is not actively transported. An increase in dansyl-galactoside fluorescence is observed upon addition of D-lactate. The fluorescence increase is not observed in membrane vesicles lacking the β-galactoside transport system, and is blocked or rapidly reversed by addition of β-galactosides, sulfhydryl reagents, inhibitors of D-lactate oxidation, or uncoupling agents. The fluorescence increase exhibits an emission maximum at 500 nm and excitation maxima at 345 nm and at 292 nm. The latter excitation maximum is absent unless D-lactate is added, indicating that the bound dansyl-galactoside molecules are excited by energy transfer from the membrane proteins. Titration of vesicles with dansyl-galactoside in the presence of D-lactate demonstrates that the β-galactoside carrier protein represents about 3.3% of the total membrane protein. The data indicate that D-lactate oxidation leads to binding of the fluorescent galactoside to the β-galactoside carrier protein in such a manner that the dansyl group is transferred to a hydrophobic environment within the membrane.
机译:荧光半乳糖苷,2-(N-丹磺酰基)-氨基乙基β-D-硫代半乳糖苷(丹磺酰基-半乳糖苷)竞争性地抑制大肠杆菌的膜小泡对乳糖的转运,但没有被主动转运。加入D-乳酸酯后,丹酰-半乳糖苷荧光增加。在缺少β-半乳糖苷转运系统的膜囊泡中未观察到荧光增加,并且通过添加β-半乳糖苷,巯基试剂,D-乳酸氧化抑制剂或解偶联剂而被阻止或迅速逆转。荧光增加在500 nm处显示最大发射,在345 nm和292 nm处显示最大激发。除非添加D-乳酸,否则不存在后者的最大激发,这表明结合的丹磺酰基-半乳糖苷分子是通过从膜蛋白的能量转移而被激发的。在D-乳酸存在下用丹磺酰基-半乳糖苷滴定小泡表明,β-半乳糖苷载体蛋白约占总膜蛋白的3.3%。数据表明D-乳酸的氧化导致荧光半乳糖苷与β-半乳糖苷载体蛋白的结合,使得丹磺酰基被转移到膜内的疏水环境中。

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