A novel gene-fusing vector: construction of a 5-GGmCC-specific chimeric methyltransferase, M.BspRI/M.BsuRI

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A vector was designed to allow predetermined and precise fusion between two cloned genes by constructing a cassette with two unique class-IIS restriction sites, 5'-ACCTGC-3' (BspMI) and 5'-CCGGATG-3' (FokI overlapping with MspI), arranged back-to-back in a divergent manner and inserted at the HincII site of a multiple cloning site (MCS) in plasmid pUC18 or analogous vehicle. Two DNA fragments or genes to be precisely fused are cloned into the MCS parts located on each side of the cassette containing the two unique class-IIS restriction sites. The BspMI and MspI/FokI sites are used to generate unidirectional deletions of the genes as previously described [Hasan et al., Gene 50 (1986) 55-62; Posfai and Szybalski, Nucleic Acids Res. 16 (1988) 6245]. The precisely trimmed genes are ligated after the cassette containing the unique class-IIS restriction sites are excised with BspMI+ FokI and the termini were blunted with mung-bean nuceleast. This method was used to construct a hybrid methyltransferase (MTase) from the M. BspRI and M. BsuRI MTases, which share a high degree of overall homology (about 65%) and have the identical sequence specificity (5'-GGmCC-3'). A hybrid MTase composed of the N-terminal part of M . BspRI and the C-terminal part of M . BsuRI was constructed and found to be fully functional.
Publisher
ELSEVIER SCIENCE BV
Issue Date
1991-04
Language
English
Article Type
Article
Keywords

MODIFICATION METHYLASE GENE; BACILLUS-SPHAERICUS R; DNA-METHYLTRANSFERASES; RECOGNITION SEQUENCE; RESTRICTION ENZYME; SPECIFICITY; SPR

Citation

GENE, v.100, pp.45 - 50

ISSN
0378-1119
DOI
10.1016/0378-1119(91)90348-F
URI
http://hdl.handle.net/10203/67343
Appears in Collection
BS-Journal Papers(저널논문)
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