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识别变形菌纲β亚类氨氧化菌AmoB蛋白的多克隆抗体。

Polyclonal antibodies recognizing the AmoB protein of ammonia oxidizers of the beta-subclass of the class Proteobacteria.

作者信息

Pinck C, Coeur C, Potier P, Bock E

机构信息

Institut für Allgemeine Botanik, Universität Hamburg, D-22609 Hamburg, Germany.

出版信息

Appl Environ Microbiol. 2001 Jan;67(1):118-24. doi: 10.1128/AEM.67.1.118-124.2001.

Abstract

A 41-kDa protein of Nitrosomonas eutropha was purified, and the N-terminal amino acid sequence was found to be nearly identical with the sequence of AmoB, a subunit of ammonia monooxygenase. This protein was used to develop polyclonal antibodies, which were highly specific for the detection of the four genera of ammonia oxidizers of the beta-subclass of Proteobacteria (Nitrosomonas, including Nitrosococcus mobilis, which belongs phylogenetically to Nitrosomonas; Nitrosospira; Nitrosolobus; and Nitrosovibrio). In contrast, the antibodies did not react with ammonia oxidizers affiliated with the gamma-subclass of Proteobacteria (Nitrosococcus oceani and Nitrosococcus halophilus). Moreover, methane oxidizers (Methylococcus capsulatus, Methylocystis parvus, and Methylomonas methanica) containing the related particulate methane monooxygenase were not detected. Quantitative immunoblot analysis revealed that total cell protein of N. eutropha consisted of approximately 6% AmoB, when cells were grown using standard conditions (mineral medium containing 10 mM ammonium). This AmoB amount was shown to depend on the ammonium concentration in the medium. About 14% AmoB of total protein was found when N. eutropha was grown with 1 mM ammonium, whereas 4% AmoB was detected when 100 mM ammonium were used. In addition, the cellular amount of AmoB was influenced by the absence of the substrate. Cells starved for more than 2 months contained nearly twice as much AmoB as actively growing cells, although these cells possessed low ammonia-oxidizing activity. AmoB was always present and could even be detected in cells of Nitrosomonas after 1 year of ammonia starvation.

摘要

纯化了嗜中性亚硝化单胞菌的一种41 kDa蛋白,发现其N端氨基酸序列与氨单加氧酶的一个亚基AmoB的序列几乎相同。用该蛋白制备了多克隆抗体,这些抗体对检测变形菌β亚类的四个氨氧化菌属(亚硝化单胞菌属,包括在系统发育上属于亚硝化单胞菌属的运动亚硝化球菌;亚硝化螺菌属;亚硝化叶菌属;亚硝化弧菌属)具有高度特异性。相比之下,这些抗体与属于变形菌γ亚类的氨氧化菌(海洋亚硝化球菌和嗜盐亚硝化球菌)不发生反应。此外,未检测到含有相关颗粒甲烷单加氧酶的甲烷氧化菌(荚膜甲基球菌、细小甲基孢囊菌和甲基单胞菌)。定量免疫印迹分析表明,在标准条件下(含有10 mM铵的矿物培养基)培养细胞时,嗜中性亚硝化单胞菌的总细胞蛋白中约6%为AmoB。结果表明,AmoB的含量取决于培养基中的铵浓度。当嗜中性亚硝化单胞菌在1 mM铵的条件下生长时,发现总蛋白中约14%为AmoB,而当使用100 mM铵时,检测到4%的AmoB。此外,AmoB的细胞含量受底物缺失的影响。饥饿超过2个月的细胞所含的AmoB几乎是活跃生长细胞的两倍,尽管这些细胞的氨氧化活性较低。AmoB始终存在,甚至在氨饥饿1年后仍可在亚硝化单胞菌的细胞中检测到。

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