pPAC-ResQ: A yeast-bacterial shuttle vector for capturing inserts from P1 and PAC clones by recombinogenic targeted cloning

Jaya Bhargava; Cooduvalli S. Shashikant; Janet L. Carr; Kevin L. Bentley; Chris T. Amemiya; Frank H. Ruddle

doi:10.1006/geno.1998.5710

pPAC-ResQ: A yeast-bacterial shuttle vector for capturing inserts from P1 and PAC clones by recombinogenic targeted cloning

Jaya Bhargava, Cooduvalli S. Shashikant, Janet L. Carr, Kevin L. Bentley, Chris T. Amemiya, Frank H. Ruddle

Research output: Contribution to journal › Article › peer-review

9 Scopus citations

Abstract

We have developed a method to capture inserts from P1 and P1 artificial chromosome (PAC) clones into a yeast-bacteria shuttle vector by using recombinogenic targeting. We have engineered a vector, pPAC-ResQ, a derivative of pClasper, which was previously used to capture inserts from yeast artificial chromosome clones, pPAC-ResQ contains DNA fragments flanking the inserts in P1 and PAC vectors as recombinogenic ends. When linearized pPAC-ResQ vector and P1 or PAC DNA are cotransformed into yeast, recombination between the two leads to the transfer of inserts into pPAC- ResQ. pPAC-ResQ clones thus obtained can be further modified in yeast for functional analysis and shuttled to Escherichia coli to produce large quantities of cloned DNA. This approach provides a rapid method to modify P1/PAC clones for functional analysis.

Original language	English (US)
Pages (from-to)	337-339
Number of pages	3
Journal	Genomics
Volume	56
Issue number	3
DOIs	https://doi.org/10.1006/geno.1998.5710
State	Published - Mar 15 1999

All Science Journal Classification (ASJC) codes

Genetics

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10.1006/geno.1998.5710

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@article{7fb3837eed0a435eb1986cf036bfec2a,

title = "pPAC-ResQ: A yeast-bacterial shuttle vector for capturing inserts from P1 and PAC clones by recombinogenic targeted cloning",

abstract = "We have developed a method to capture inserts from P1 and P1 artificial chromosome (PAC) clones into a yeast-bacteria shuttle vector by using recombinogenic targeting. We have engineered a vector, pPAC-ResQ, a derivative of pClasper, which was previously used to capture inserts from yeast artificial chromosome clones, pPAC-ResQ contains DNA fragments flanking the inserts in P1 and PAC vectors as recombinogenic ends. When linearized pPAC-ResQ vector and P1 or PAC DNA are cotransformed into yeast, recombination between the two leads to the transfer of inserts into pPAC- ResQ. pPAC-ResQ clones thus obtained can be further modified in yeast for functional analysis and shuttled to Escherichia coli to produce large quantities of cloned DNA. This approach provides a rapid method to modify P1/PAC clones for functional analysis.",

author = "Jaya Bhargava and Shashikant, {Cooduvalli S.} and Carr, {Janet L.} and Bentley, {Kevin L.} and Amemiya, {Chris T.} and Ruddle, {Frank H.}",

note = "Funding Information: We thank Asaf Halevi, Hirohide Kawasaki, and Wayne Wang for technical assistance and Chang Bae Kim for providing the PAC-13B clone. This work was supported by grants to F.H.R. (NIH-GM 09966; NSF IBN-9630567) and to C.T.A. (NIH-AI39008-03; NSF IBN-9614940).",

year = "1999",

month = mar,

day = "15",

doi = "10.1006/geno.1998.5710",

language = "English (US)",

volume = "56",

pages = "337--339",

journal = "Genomics",

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publisher = "Academic Press Inc.",

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T2 - A yeast-bacterial shuttle vector for capturing inserts from P1 and PAC clones by recombinogenic targeted cloning

AU - Bhargava, Jaya

AU - Shashikant, Cooduvalli S.

AU - Carr, Janet L.

AU - Bentley, Kevin L.

AU - Amemiya, Chris T.

AU - Ruddle, Frank H.

N1 - Funding Information: We thank Asaf Halevi, Hirohide Kawasaki, and Wayne Wang for technical assistance and Chang Bae Kim for providing the PAC-13B clone. This work was supported by grants to F.H.R. (NIH-GM 09966; NSF IBN-9630567) and to C.T.A. (NIH-AI39008-03; NSF IBN-9614940).

PY - 1999/3/15

Y1 - 1999/3/15

N2 - We have developed a method to capture inserts from P1 and P1 artificial chromosome (PAC) clones into a yeast-bacteria shuttle vector by using recombinogenic targeting. We have engineered a vector, pPAC-ResQ, a derivative of pClasper, which was previously used to capture inserts from yeast artificial chromosome clones, pPAC-ResQ contains DNA fragments flanking the inserts in P1 and PAC vectors as recombinogenic ends. When linearized pPAC-ResQ vector and P1 or PAC DNA are cotransformed into yeast, recombination between the two leads to the transfer of inserts into pPAC- ResQ. pPAC-ResQ clones thus obtained can be further modified in yeast for functional analysis and shuttled to Escherichia coli to produce large quantities of cloned DNA. This approach provides a rapid method to modify P1/PAC clones for functional analysis.

AB - We have developed a method to capture inserts from P1 and P1 artificial chromosome (PAC) clones into a yeast-bacteria shuttle vector by using recombinogenic targeting. We have engineered a vector, pPAC-ResQ, a derivative of pClasper, which was previously used to capture inserts from yeast artificial chromosome clones, pPAC-ResQ contains DNA fragments flanking the inserts in P1 and PAC vectors as recombinogenic ends. When linearized pPAC-ResQ vector and P1 or PAC DNA are cotransformed into yeast, recombination between the two leads to the transfer of inserts into pPAC- ResQ. pPAC-ResQ clones thus obtained can be further modified in yeast for functional analysis and shuttled to Escherichia coli to produce large quantities of cloned DNA. This approach provides a rapid method to modify P1/PAC clones for functional analysis.

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pPAC-ResQ: A yeast-bacterial shuttle vector for capturing inserts from P1 and PAC clones by recombinogenic targeted cloning

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