Cloning and expression of human defensin HNP-1 genomic DNA in Escherichia coli

被引：4

作者：

Takemura, H

Kaku, M

Kohno, S

Tanaka, H

Yoshida, R

Ishida, K

Mizukane, R

Koga, H

Hara, K

Usui, T

Ezaki, T

机构：

[1] NAGASAKI UNIV,SCH MED,DEPT INTERNAL MED 2,NAGASAKI 852,JAPAN

[2] GIFU UNIV,SCH MED,DEPT MICROBIOL,GIFU 500,JAPAN

来源：

JOURNAL OF MICROBIOLOGICAL METHODS | 1996年 / 25卷 / 03期

关键词：

cloning; defensin; Escherichia coli; expression; HNP-1; gene; pGEX-2T;

D O I：

10.1016/0167-7012(95)00103-4

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

We amplified a 181-bp DNA fragment encoding HNP-1 from genomic DNA of human polymorphonucleated neutrophils by PCR. Sequencing of this fragment revealed that it only contained the mature protein coding region of HNP-1 and no intron was found in the sequences. The PCR product of HNP-1 genomic DNA was then cloned and expressed in Escherichia coli as a fusion protein with Schistosoma japonicum glutathione S-transferase (the GST-HNP-1 fusion protein). The GST-HNP-1 fusion protein was expressed as insoluble inclusion bodies, so they were collected and solubilized in 8 M urea. Thus, reasonably pure GST-HNP-1 fusion protein was obtained, with which rabbits were immunized to raise polyclonal antibody against HNP-1. Ouchterlony immunodiffusion and immunoblotting showed that the antiserum reacted with chemically synthesized HNP-1, -2 and human PMN extracts and did not cross react with human GST in these assays. We demonstrated that human defensin HNP-1, a small cationic protein, was expressed in E. coli as an insoluble GST fusion protein, and polyclonal antibody raised by immunizing rabbits with this fusion protein did not cross react with human GST and was specific to defensins.

引用

页码：287 / 293

页数：7

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