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Literature DB >> 9628365

Does BcgI, a unique restriction endonuclease, require two recognition sites for cleavage?

Abstract

BcgI is a multi-subunit restriction-modification (R-M) complex. BcgI prefers pBR322 DNA over pUC19 in a DNA cleavage reaction. Linearized pBR322 contains two BcgI recognition sites and pUC19 has only one site. To test whether two target sites are required for BcgI cleavage, one of the two sites in pBR322 was deleted, and as a result pBR322-1 became a poor substrate for BcgI. Conversely, adding a BcgI site to pUC19 makes it a much better substrate for BcgI cleavage. In addition, the BcgI (R-M) complex forms a heterohexamer in solution that is capable of interacting with two recognition sites. Our results suggest that BcgI requires two recognition sites for cleavage.

Entities: Chemical

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Year: 1998 PMID： 9628365

Source DB: PubMed Journal: Biol Chem ISSN： 1431-6730 Impact factor: 3.915

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Cited

12 in total

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Authors: T Berge; D J Ellis; D T Dryden; J M Edwardson; R M Henderson
Journal: Biophys J Date: 2000-07 Impact factor: 4.033

2. Engineering a nicking endonuclease N.AlwI by domain swapping.

Authors: Y Xu; K D Lunnen; H Kong
Journal: Proc Natl Acad Sci U S A Date: 2001-10-30 Impact factor: 11.205

3. One recognition sequence, seven restriction enzymes, five reaction mechanisms.

Authors: Darren M Gowers; Stuart R W Bellamy; Stephen E Halford
Journal: Nucleic Acids Res Date: 2004-06-29 Impact factor: 16.971

Review 4. Type II restriction endonucleases--a historical perspective and more.

Authors: Alfred Pingoud; Geoffrey G Wilson; Wolfgang Wende
Journal: Nucleic Acids Res Date: 2014-05-30 Impact factor: 16.971

5. Bacteriophage T4 endonuclease II, a promiscuous GIY-YIG nuclease, binds as a tetramer to two DNA substrates.

Authors: Pernilla Lagerbäck; Evalena Andersson; Christer Malmberg; Karin Carlson
Journal: Nucleic Acids Res Date: 2009-08-07 Impact factor: 16.971

6. TstI, a Type II restriction-modification protein with DNA recognition, cleavage and methylation functions in a single polypeptide.

Authors: Rachel M Smith; Christian Pernstich; Stephen E Halford
Journal: Nucleic Acids Res Date: 2014-03-14 Impact factor: 16.971

Does BcgI, a unique restriction endonuclease, require two recognition sites for cleavage?

1. Translocation-independent dimerization of the EcoKI endonuclease visualized by atomic force microscopy.

2. Engineering a nicking endonuclease N.AlwI by domain swapping.

3. One recognition sequence, seven restriction enzymes, five reaction mechanisms.

Review 4. Type II restriction endonucleases--a historical perspective and more.

5. Bacteriophage T4 endonuclease II, a promiscuous GIY-YIG nuclease, binds as a tetramer to two DNA substrates.

6. TstI, a Type II restriction-modification protein with DNA recognition, cleavage and methylation functions in a single polypeptide.

7. Organization of the BcgI restriction-modification protein for the transfer of one methyl group to DNA.

8. Organization of the BcgI restriction-modification protein for the cleavage of eight phosphodiester bonds in DNA.

Review 9. Restriction endonucleases: classification, properties, and applications.

10. Concerted action at eight phosphodiester bonds by the BcgI restriction endonuclease.