Cloning and expressing of a harpin-encoding gene from Pseudomonas syringae pv. Glycinea
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Supported by the Foundation of Jilin Science and Technology Development Plan(20060204-02), the Ministry of Agriculture, "Eleventh Five-Year" genetically modified organisms to cultivate new varieties of major projects(2008ZX08003-004) and the Project Spon

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    Abstract:

    Abstract: [Methods, objective] We amplified the 1026 bp hrp(hypersensitive response and pathogenicity ) gene from Pseudomonas syringae pv. glycinea isolate Psg12 genomic DNA by PCR technique, and then constructed expression vector pGEX-hrpZPsg12 with regular molecular cloning operation. The recombinant plasmid was transformed into BL21(DE3). Recombinant protein was induced by Isopropylthio-β-D-Galacgoside (IPTG).[Results] The molecular mass of the fusion protein is 61kDa analyzed by SDS-PAGE. The protein, similar to the other known harpins, was heat-stable, which contained abundant glycine(G), but had no cysteine. Furthermore, this protein was sensitive to protease K and able to trigger hypersensitive response (HR) in common tobacco. The HR elicitation by the protein in tobacco was inhibited by eukayotic metabolic inhibitors, NH4VO3 and LaCl3. The hrpZ gene showed 79% identity to hrpZPsg which cloned from P. syringae pv. glycinea(Psg r0) in Japan and 79-99% identity to other hrpZ in GenBank. However, it did not show any sequence identity with those of other genus of gram-negative plant pathogenic bacteria. [Conclusion] In summary, hrpZPsg12 was a novel gene that was cloned by us from P. syringae pv. glycinea, and this is the first report to express hrpZPsg12 gene in BL21.

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Zhaoyuan Jiang, Xiaowei Zou, Jie Gao, Qingrong Bai, Jiahuan Zhang. Cloning and expressing of a harpin-encoding gene from Pseudomonas syringae pv. Glycinea. [J]. Acta Microbiologica Sinica, 2009, 49(10): 1403-1407

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History
  • Received:March 20,2009
  • Revised:May 06,2009
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  • Online: March 13,2012
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