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关于质子动力在变形链球菌DR0001菌株的葡萄糖 - 磷酸烯醇丙酮酸磷酸转移酶活性缺陷突变体转运葡萄糖过程中所起作用的证据。

Evidence for the involvement of proton motive force in the transport of glucose by a mutant of Streptococcus mutans strain DR0001 defective in glucose-phosphoenolpyruvate phosphotransferase activity.

作者信息

Hamilton I R, St Martin E J

出版信息

Infect Immun. 1982 May;36(2):567-75. doi: 10.1128/iai.36.2.567-575.1982.

Abstract

Streptococcus mutans DR0001 and a glucose-phosphotransferase (PTS)-defective mutant, DR0001/6, were grown anaerobically in a chemostat with a glucose limitation at dilution rates (D) of 0.04 to 0.6 h(-1) (mean generation time, 17 to 1.2 h). The mutant possessed only 15% of glucose-PTS activity of the wild type and gave cell yields (19%) less than those of the wild type. Glucose-PTS activity in strains DR0001 was maximum at D = 0.1 h(-1) and was adequate to account for transport in the chemostat at all dilution rates except D = 0.6 h(-1), at which it was 80% of the actual glucose uptake activity. The mutant DR0001/6, on the other hand, possessed only sufficient glucose-PTS activity to sustain growth at below D = 0.1 h(-1), indicating the presence of an alternate transport activity. This was confirmed in glycolytic rate experiments with washed cells, which demonstrated that the mutant showed rates 11- to 27-fold higher than that accountable via glucose-PTS activity alone. The wild-type organism contained both a high (K(s), 6.7 to 8.0 muM)- and a low (K(s), 57 to 125 muM)-affinity transport system, whereas the glucose-PTS-defective mutant contained only the low-affinity system (K(s), 62 to 133 muM). The glucose-PTS was shown to be the high-affinity system. Glucose uptake by the mutant was unaffected by 8 mM sodium arsenate, 10 mM azide, and 10 mM dinitrophenol but was completely inhibited by 0.05 mM sodium iodoacetate. Glycolysis in the organism was almost completely inhibited by 0.25 mM N',N' -dicyclohexylcarbodiimide (DCCD), indicating the involvement of an ATPase in glucose uptake. The ionophores carbonylcyanide-m-chlorophenylhydrazone and tetrachlorosali-cylanilide were inhibitory at concentrations of 10 muM, suggesting that a proton gradient was important in the transport process. Higher levels of DCCD and the ionophores were required to inhibit the wild-type organism to the same degree. A mechanism is proposed for the alternative transport system whereby proton motive force is created by the extrusion of protons by the DCCD-sensitive ATPase and glucose is transported down a proton gradient in a symport with protons.

摘要

变形链球菌DR0001和一株葡萄糖磷酸转移酶(PTS)缺陷型突变体DR0001/6在恒化器中进行厌氧培养,葡萄糖受限,稀释率(D)为0.04至0.6 h⁻¹(平均世代时间为17至1.2小时)。该突变体的葡萄糖-PTS活性仅为野生型的15%,细胞产量(19%)低于野生型。菌株DR0001中的葡萄糖-PTS活性在D = 0.1 h⁻¹时最高,除D = 0.6 h⁻¹外,在所有稀释率下都足以解释恒化器中的转运情况,在D = 0.6 h⁻¹时,其活性为实际葡萄糖摄取活性的80%。另一方面,突变体DR0001/6仅具有足够的葡萄糖-PTS活性以维持低于D = 0.1 h⁻¹的生长,这表明存在替代转运活性。这在洗涤细胞的糖酵解速率实验中得到证实,该实验表明突变体的速率比仅通过葡萄糖-PTS活性所能解释的速率高11至27倍。野生型生物体同时含有高亲和力(Kₛ,6.7至8.0 μM)和低亲和力(Kₛ,57至125 μM)转运系统,而葡萄糖-PTS缺陷型突变体仅含有低亲和力系统(Kₛ,62至133 μM)。葡萄糖-PTS被证明是高亲和力系统。突变体对葡萄糖的摄取不受8 mM砷酸钠、10 mM叠氮化物和10 mM二硝基苯酚的影响,但被0.05 mM碘乙酸钠完全抑制。生物体中的糖酵解几乎被0.25 mM N',N'-二环己基碳二亚胺(DCCD)完全抑制,表明一种ATP酶参与了葡萄糖摄取。离子载体羰基氰化物间氯苯腙和四氯水杨酰苯胺在浓度为10 μM时具有抑制作用,这表明质子梯度在转运过程中很重要。需要更高水平的DCCD和离子载体才能将野生型生物体抑制到相同程度。提出了一种替代转运系统的机制,即由DCCD敏感的ATP酶将质子挤出产生质子动力,葡萄糖在与质子的同向转运中顺着质子梯度进行转运。

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