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Molecular cloning of haemoglobin-binding protein HgbA in the outer membrane of Actinobacillus pleuropneumoniae

机译:Actinobacillus胸膜外膜中血红蛋白结合蛋白HGBA的分子克隆

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From the porcine pathogen Actinobacillus pleuropneumoniae cultivated in iron-deficient or haem-deficient media, haemoglobin (Hb)-agarose affinity purification was exploited to isolate an outer-membrane protein of ~105?kDa, designated HgbA. Internal peptide sequences of purified HgbA were used to design oligonucleotide primers for PCR amplification, yielding amplicons that showed partial sequences with homology to hgbA of Pasteurella multocida. Upon screening two genomic libraries of A. pleuropneumoniae serotype 1 strain 4074, positive clones were assembled into an ORF of 2838?bp. HgbA (946?aa) includes a signal peptide of 23?aa and the deduced HgbA sequence (104?890?Da) also demonstrated a possible Ton box. The promoter region of hgbA from A. pleuropneumoniae serotype 1 showed consensus for ?35 and ?10 sequences and a putative Fur-binding site. RT-PCR confirmed that hgbA of A. pleuropneumoniae is upregulated in response to diminished levels of iron in the culture medium. While an internally deleted hgbA mutant was unable to use pig Hb as sole source of iron for growth, flow cytometry confirmed its Hb binding; the internally deleted sequences may not be required for Hb binding, but appear necessary for the iron supply from Hb. HgbA is required for growth of A. pleuropneumoniae in the presence of Hb as sole iron source.
机译:从缺铁或血管培养的猪病原体Actinobacillus胸膜肺炎,血红蛋白(Hb) - 血红素亲和纯化被利用以分离〜105Ωkda的外膜蛋白,指定HGBA。纯化HGBA的内部肽序列用于设计PCR扩增的寡核苷酸引物,产生与帕斯特氏藻菌的HGBA具有同源性的偏序列的扩增子。在筛选A.Pleuropneumoniae血清型1株4074的两个基因组文库后,将阳性克隆组装成2838μlβBp。 HGBA(946?AA)包括23〜A的信号肽和推导的HGBA序列(104?890?DA)也表现出了可能的吨盒。来自A.Pleuropneumoniae血清型1的HGBA的启动子区显示出α35和α15和序列的共识和推定的毛皮结合位点。 RT-PCR证实A.Pleuropneumoniae的HGBA是响应于培养基中的铁水平减少的。虽然内部删除的HGBA突变体无法使用猪Hb作为生长的唯一的铁来源,但流式细胞仪证实其Hb结合; Hb结合可能不需要内部删除的序列,但是从Hb的铁供应所需的表现出来。 HGBA是在HB的存在下的胸膜肺源存在下胸膜炎的生长所必需的。

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