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Literature DB >> 20857241

pYEMF, a pUC18-derived XcmI T-vector for efficient cloning of PCR products.

Abstract

A 1330-bp DNA sequence with two XcmI cassettes was inserted into pUC18 to construct an efficient XcmI T-vector parent plasmid, pYEMF. The large size of the inserted DNA fragment improved T-vector cleavage efficiency, and guaranteed good separation of the molecular components after restriction digestion. The pYEMF-T-vector generated from parent plasmid pYEMF permits blue/white colony screening; cloning efficiency analysis showed that most white colonies (>75%) were putative transformants which carried the cloning product. The sequence analysis and design approach presented here will facilitate applications in the fields of molecular biology and genetic engineering.

Mesh：

Substances：

Year: 2011 PMID： 20857241 DOI： 10.1007/s12033-010-9333-y

Source DB: PubMed Journal: Mol Biotechnol ISSN： 1073-6085 Impact factor: 2.695

16 in total

1. XcmI site-containing vector for direct cloning and in vitro transcription of PCR product.

Authors: N Arashi-Heese; M Miwa; H Shibata
Journal: Mol Biotechnol Date: 1999-10 Impact factor: 2.695

2. A universal method for the direct cloning of PCR amplified nucleic acid.

Authors: D A Mead; N K Pey; C Herrnstadt; R A Marcil; L M Smith
Journal: Biotechnology (N Y) Date: 1991-07

3. Construction of T-vectors, a rapid and general system for direct cloning of unmodified PCR products.

Authors: D Marchuk; M Drumm; A Saulino; F S Collins
Journal: Nucleic Acids Res Date: 1991-03-11 Impact factor: 16.971

4. A simple and efficient method for direct cloning of PCR products using ddT-tailed vectors.

Authors: T A Holton; M W Graham
Journal: Nucleic Acids Res Date: 1991-03-11 Impact factor: 16.971

5. General method for direct cloning of DNA fragments generated by the polymerase chain reaction.

Authors: D Kovalic; J H Kwak; B Weisblum
Journal: Nucleic Acids Res Date: 1991-08-25 Impact factor: 16.971

6. One-step preparation of a TA-cloning vector from a specially designed parent plasmid containing a dual lacZ gene system.

Authors: Soo Youn Jun; Seong Jun Yoon; Sang Hyeon Kang
Journal: Mol Biotechnol Date: 2010-05 Impact factor: 2.695

7. pUCPCR1. A vector for direct cloning of PCR products in a double Xcm1 restriction site offering compatible single 3'-overhanging T residues.

Authors: E de Vries
Journal: Mol Biotechnol Date: 1998-12 Impact factor: 2.695

pYEMF, a pUC18-derived XcmI T-vector for efficient cloning of PCR products.

1. XcmI site-containing vector for direct cloning and in vitro transcription of PCR product.

2. A universal method for the direct cloning of PCR amplified nucleic acid.

3. Construction of T-vectors, a rapid and general system for direct cloning of unmodified PCR products.

4. A simple and efficient method for direct cloning of PCR products using ddT-tailed vectors.

5. General method for direct cloning of DNA fragments generated by the polymerase chain reaction.

6. One-step preparation of a TA-cloning vector from a specially designed parent plasmid containing a dual lacZ gene system.

7. pUCPCR1. A vector for direct cloning of PCR products in a double Xcm1 restriction site offering compatible single 3'-overhanging T residues.

8. Cloning unmodified PCR products using engineered XcmI restriction sites in a portable cassette.

9. XcmI-containing vector for direct cloning of PCR products.

10. A versatile zero background T-vector system for gene cloning and functional genomics.

1. pPCV, a versatile vector for cloning PCR products.

2. pELMO, an optimised in-house cloning vector.

3. A novel binary T-vector with the GFP reporter gene for promoter characterization.

4. pXST, a novel vector for TA cloning and blunt-end cloning.