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Matrix-Assisted Laser Desorption/Ionization Time-of-Flight (MALDI-TOF)- Based Cloning of Enolase, ENO1, from Cryphonectria parasitica  

Kim, Myoung-Ju (Institute for Molecular Biology and Genetics, Basic Science Research Institute, Chonbuk National University)
Chung, Hea-Jong (Institute for Molecular Biology and Genetics, Basic Science Research Institute, Chonbuk National University)
Park, Seung-Moon (Institute for Molecular Biology and Genetics, Basic Science Research Institute, Chonbuk National University)
Park, Sung-Goo (Korea Research Institute of Bioscience and Biotechnology)
Chung, Dae-Kyun (School of Biotechnology and Institute of Life Science and Resources, Kyung Hee University)
Yang, Moon-Sik (Institute for Molecular Biology and Genetics, Basic Science Research Institute, Chonbuk National University)
Kim, Dae-Hyuk (Institute for Molecular Biology and Genetics, Basic Science Research Institute, Chonbuk National University)
Publication Information
Journal of Microbiology and Biotechnology / v.14, no.3, 2004 , pp. 620-627 More about this Journal
Abstract
On the foundation of a database of genome sequences and protein analyses, the ability to clone a gene based on a peptide analysis is becoming more feasible and effective for identifying a specific gene and its protein product of interest. As such, the current study conducted a protein analysis using 2-D PAGE followed by MALDI- TOF and ESI-MS to identify a highly expressed gene product of C. parasitica. A distinctive and highly expressed protein spot with a molecular size of 47.2 kDa was randomly selected and MALDI-TOF MS analysis was conducted. A homology search indicated that the protein appeared to be a fungal enolase (enol). Meanwhile, multiple alignments of fungal enolases revealed a conserved amino acid sequence, from which degenerated primers were designed. A screening of the genomic $\lambda$ library of C. parasitica, using the PCR amplicon as a probe, was conducted to obtain the full-length gene, while RT-PCR was performed for the cDNA. The E. coli-expressed eno 1 exhibited enolase enzymatic activity, indicating that the cloned gene encoded the C. parasitica enolase. Moreover, ESI-MS of two of the separated peptides resolved from the protein spot on 2-D PAGE revealed sequences identical to the deduced sequences, suggesting that the cloned gene indeed encoded the resolved protein spot. Northern blot analysis indicated a consistent accumulation of an eno1 transcript during the cultivation.
Keywords
C. parasitica; enolase; 2-D PAGE; MALDI- TOF; ESI-MS;
Citations & Related Records
Times Cited By KSCI : 1  (Citation Analysis)
Times Cited By Web Of Science : 7  (Related Records In Web of Science)
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