Cloning and expression of ornithine decarboxylase gene from human colorectal carcinoma

doi:10.3748/wjg.v9.i4.714

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Apr 15, 2003 (publication date) through Nov 8, 2024

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World Journal of Gastroenterology

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1007-9327

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Baishideng Publishing Group Inc, 7041 Koll Center Parkway, Suite 160, Pleasanton, CA 94566, USA

Colorectal Cancer

World J Gastroenterol. Apr 15, 2003; 9(4): 714-716
Published online Apr 15, 2003. doi: 10.3748/wjg.v9.i4.714

Cloning and expression of ornithine decarboxylase gene from human colorectal carcinoma

Hai-Yan Hu, Xian-Xi Liu, Chun-Ying Jiang, Yan Zhang, Ji-Feng Bian, Yi Lu, Zhao Geng, Shi-Lian Liu, Chuan-Hua Liu, Xiao-Ming Wang, Wei Wang

Hai-Yan Hu, Xian-Xi Liu, Ji-Feng Bian, Yi Lu, Shi-Lian Liu, Chuan-Hua Liu, Xiao-Ming Wang, Yan Zhang, Wei Wang, Geng Zhao, Experimental Centre of Medical Molecular Biology, School of Medicine, Shandong University, Jinan 250012, Sandong Province, China

Chun-Ying Jiang, Department of colo-proctology, The affiliated Hospital of Shandong University of Tradition Chinese Medicine, Jinan 250012, Sandong Province, China

Author contributions: All authors contributed equally to the work.

Supported by Scientific Research Fund of national Ministry of Health, No.98-1-173

Correspondence to: Xian-Xi Liu, Experimental Centre of Medical Molecular Biology, School of Medicine, Shandon University, Jinan 250012, Shandong Province, China. xianxi@sdu.edu.cn

Telephone: +86-531-8382346

Received: July 4, 2002
Revised: October 24, 2002
Accepted: October 31, 2002
Published online: April 15, 2003

Abstract

AIM: To construct and express ODC recombinant gene for further exploring its potential use in early diagnosis of colorectal carcinoma.

METHODS: Total RNA was extracted from colon cancer tissues and amplified by reverse-transcription PCR with two primers, which span the whole coding region of ODC. The synthesized ODC cDNA was cloned into vector pQE-30 at restriction sites BamH I and Sal I which constituted recombinant expression plasmid pQE30-ODC. The sequence of inserted fragment was confirmed by DNA sequencing, the fusion protein including 6His-tag was facilitated for purification by Ni-NTA chromatographic column.

RESULTS: ODC expression vector was constructed and confirmed with restriction enzyme digestion and subsequent DNA sequencing. The DNA sequence matching on NCBI Blast showed 99% affinity. The vector was transformed into E. coli M15 and expressed. The expressed ODC protein was verified with Western blotting.

CONCLUSION: The ODC prokaryote expression vector is constructed and thus greatly facilitates to study the role of ODC in colorectal carcinoma.

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