首页> 外文期刊>Journal of bacteriology >Cloning and sequencing of a Moraxella bovis pilin gene.
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Cloning and sequencing of a Moraxella bovis pilin gene.

机译:牛莫拉氏菌菌毛蛋白基因的克隆和测序。

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Moraxella bovis pili have been shown to play a major role in both infectivity and protective immunity of bovine infectious keratoconjunctivitis. Sonicated M. bovis DNA from the piliated strain EPP63 was inserted into the vector lambda gt11 with EcoRI linkers. Recombinant phage were screened with an oligonucleotide probe based on the amino-terminal portion of the DNA sequence of a Neisseria gonorrhoeae pilin gene. Two candidate phages produced a protein that comigrated with EPP63 beta pilin in sodium dodecyl sulfate-polyacrylamide gels and bound anti-pilus antisera. The 1.9-kilobase insert from one of these, lambda gt11M182, was subcloned in both orientations into pBR322, forming the plasmids pMxB7 and pMxB9, both of which produced beta pilin, as did pMxB12, a HindIII deletion derivative of pMxB7. In HB101(pMxB12), the M. bovis pilin protein was shown to be primarily localized in the inner membrane. The entire 939-base-pair insert of pMxB12 was sequenced, revealing a ribosome binding site just upstream of the coding region and an AT-rich region further upstream containing some potential RNA polymerase recognition sites. The translation of the sequence predicts a six-amino-acid leader sequence preceding the phenylalanine that begins the mature protein. Codon usage analysis of the M. bovis beta pilin gene revealed greater use of the CUA codon for leucine than usual for a well-expressed Escherichia coli gene. Comparisons of the M. bovis EPP63 beta pilin protein sequence with other pilin gene sequences are presented.
机译:牛莫拉氏菌已被证明在牛传染性角膜结膜炎的传染性和保护性免疫中起主要作用。将来自菌株EPP63的超声处理的牛分枝杆菌DNA插入具有EcoRI接头的载体λgt11中。基于淋病奈瑟氏球菌菌毛蛋白基因的DNA序列的氨基末端部分,用寡核苷酸探针筛选重组噬菌体。两种候选噬菌体产生的蛋白质在十二烷基硫酸钠-聚丙烯酰胺凝胶中结合了EPP63β菌毛蛋白,并结合了抗菌毛抗血清。将其中一个λgt11M182的1.9碱基碱基插入两个方向亚克隆到pBR322中,形成质粒pMxB7和pMxB9,两者均产生β菌毛蛋白,而pMxB12(pMxB7的HindIII缺失衍生物)也产生了β菌毛。在HB101(pMxB12)中,牛分枝杆菌pilin蛋白显示主要位于内膜中。对pMxB12的整个939个碱基对的插入片段进行了测序,揭示了位于编码区上游的核糖体结合位点和位于上游的富含AT的区域,其中含有一些潜在的RNA聚合酶识别位点。该序列的翻译预测在开始成熟蛋白质的苯丙氨酸之前的六氨基酸前导序列。牛分枝杆菌βpilin基因的密码子使用分析显示,亮氨酸大肠杆菌的CUA密码子比亮氨酸的使用更多。提出了牛分枝杆菌EPP63β菌毛蛋白蛋白序列与其他菌毛蛋白基因序列的比较。

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