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脑突触小泡对谷氨酸的摄取。蛋白脂质体中转运的能量依赖性及功能重建。

Glutamate uptake by brain synaptic vesicles. Energy dependence of transport and functional reconstitution in proteoliposomes.

作者信息

Maycox P R, Deckwerth T, Hell J W, Jahn R

机构信息

Department of Neurochemistry, Max-Planck-Institute for Psychiatry, Martinsried, Federal Republic of Germany.

出版信息

J Biol Chem. 1988 Oct 25;263(30):15423-8.

PMID:2902091
Abstract

The dependence of glutamate uptake on ATP-generated proton electrochemical potential was studied in a highly purified preparation of synaptic vesicles from rat brain. At low chloride concentration (4 mM), the proton pump present in synaptic vesicles generated a large membrane potential (inside-positive), associated with only minor acidification. Under these conditions, the rate of L-[3H]glutamate uptake was maximal. In addition, L-glutamate induced acidification of the vesicle interior. D-Glutamate produced only 40% of the effect, and L-aspartate or gamma-aminobutyric acid produced less than 5%. The initial rate of glutamate-induced acidification increased with increasing glutamate concentration. It was saturable and showed first-order kinetics (KM = 0.32 mM). Correspondingly, L-glutamate induced a small reduction in the membrane potential. The rate of ATP hydrolysis was unaffected. In comparison, glutamate had no effect on acidification or membrane potential in resealed membranes of chromaffin granules. At high chloride concentration (150 mM), the vesicular proton pump generated a large pH difference, associated with a small change in membrane potential. Under these conditions, uptake of L-[3H]glutamate by synaptic vesicles was low. For reconstitution, vesicle proteins were solubilized with the detergent sodium cholate, supplemented with brain phospholipids, and incorporated into liposomes. Proton pump and glutamate uptake activities of the proteoliposomes showed properties similar to those of intact vesicles indicating that the carrier was reconstituted in a functionally active form. It is concluded that glutamate uptake by synaptic vesicles is dependent on the membrane potential and that all components required for uptake are integral parts of the vesicle membrane.

摘要

在大鼠脑突触小泡的高度纯化制剂中研究了谷氨酸摄取对ATP产生的质子电化学势的依赖性。在低氯浓度(4 mM)下,突触小泡中存在的质子泵产生了较大的膜电位(内膜为正),仅伴有轻微的酸化。在这些条件下,L-[3H]谷氨酸的摄取速率最大。此外,L-谷氨酸诱导小泡内部酸化。D-谷氨酸仅产生40%的效应,而L-天冬氨酸或γ-氨基丁酸产生的效应小于5%。谷氨酸诱导的酸化初始速率随谷氨酸浓度增加而增加。它是可饱和的,并表现出一级动力学(KM = 0.32 mM)。相应地,L-谷氨酸诱导膜电位略有降低。ATP水解速率不受影响。相比之下,谷氨酸对嗜铬颗粒重封膜的酸化或膜电位没有影响。在高氯浓度(150 mM)下,小泡质子泵产生了较大的pH差异,伴有膜电位的微小变化。在这些条件下,突触小泡对L-[3H]谷氨酸的摄取较低。为了进行重组,用去污剂胆酸钠溶解小泡蛋白,补充脑磷脂,并将其整合到脂质体中。蛋白脂质体的质子泵和谷氨酸摄取活性表现出与完整小泡相似的特性,表明载体以功能活性形式重组。结论是突触小泡对谷氨酸的摄取依赖于膜电位,摄取所需的所有成分都是小泡膜的组成部分。

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