慢生型大豆根瘤菌(Bradyrhizobium japonicum)聚羟丁酸合成酶基因(phbC)突变体的构建及其特性

通过转座子Tn5诱变和同源重组 ,构建了BradyrhizobiumjaponicumUSDA110聚羟丁酸合成酶基因 (phbC)突变体 .序列测定确定了转座子插入的精确位置 ,所获得的 4个转座子诱变的质粒其Tn5插在 phbC基因内两个相距仅 9bp的位点 .被Southern和PCR证实的突变体菌株仍能产生相当于野生型菌株 12 .97%～ 2 5 .10 %的PHB ,并且在突变体和野生型菌株总DNA杂交图上都呈现出一条约 5kb的阳性带 ,推测在B .japonicum基因组中存在不止一个聚羟丁酸合成酶基因 .图 3表 4参

Cloning,Sequencing and Characterization of 3-Hydroxybutyrate Dehydrogenase Encoding Gene(bdh A)in Bradyrhizobium japonicum USDA110 Strain

The current study describes the molecular characterization of a clone which can restore the ability of bdh A mutant strains NGRPA2 and Rm11107 to utilize 3-hydroxybutyrate as a sole carbon source (Hbu+ ). This clone was screened out by complementation experiment from Bradyrhizobium japonicum US-DAI 10 genomic library, and the presence of bdhA gene in the clone was verified by Bdh assay and Southern blot analysis. Furthermore, the entire sequence of bdhA. gene was sequenced and the sequence was deposited in GenBank database under the accession number AY077581. bdhA gene comprises 789 base pairs and encodes Bdh with 262 amino acid of MW 27.59 kDa. Interposon JlKm was inserted into the bdhA ORF at EcoR I site and the bdhA mutant was constructed in B .japonicum by homologous recombination. Plant assay result did not show obvious effects of mutation of bdhA gene on nodulation and nitrogen-fixation.