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Literature DB >> 9951708

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

Abstract

The multiple cloning site of pUC19 was replaced by a multiple cloning site possessing a double Xcm1 restriction site. Digestion with XcmI gives a linear vector with a single 3'-overhanging T-residue at both ends. This provides the easiest way of creating a vector in which PCR fragments produced by Taq polymerase can be directly cloned without further modifications.

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Year: 1998 PMID： 9951708 DOI： 10.1007/BF02740849

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

3 in total

1. 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

2. Novel non-templated nucleotide addition reactions catalyzed by procaryotic and eucaryotic DNA polymerases.

Authors: J M Clark
Journal: Nucleic Acids Res Date: 1988-10-25 Impact factor: 16.971

3. Improved M13 phage cloning vectors and host strains: nucleotide sequences of the M13mp18 and pUC19 vectors.

Authors: C Yanisch-Perron; J Vieira; J Messing
Journal: Gene Date: 1985 Impact factor: 3.688

3 in total

5 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. The PRESAT-vector: asymmetric T-vector for high-throughput screening of soluble protein domains for structural proteomics.

Authors: Natsuko Goda; Takeshi Tenno; Hirotoshi Takasu; Hidekazu Hiroaki; Masahiro Shirakawa
Journal: Protein Sci Date: 2004-03 Impact factor: 6.725

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

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

2. Novel non-templated nucleotide addition reactions catalyzed by procaryotic and eucaryotic DNA polymerases.

3. Improved M13 phage cloning vectors and host strains: nucleotide sequences of the M13mp18 and pUC19 vectors.

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

2. The PRESAT-vector: asymmetric T-vector for high-throughput screening of soluble protein domains for structural proteomics.

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

4. Generating DNA sequences encoding tandem peptide repeats suitable for expression and immunological application.

5. Development of new T-vectors containing the luciferase gene. Easy application for direct cloning of a promoter DNA.