Streamlined procedure for the production of normal and altered versions of recombinant human proinsulin

Robert B. Mackin

doi:10.1006/prep.1998.1024

Streamlined procedure for the production of normal and altered versions of recombinant human proinsulin

Robert B. Mackin

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

12 Scopus citations

Abstract

A method for the simplified, reproducible production of both normal and altered versions of human proinsulin has been developed. A polyhistidine/proinsulin fusion protein was expressed using a prokaryotic expression system and partially purified by affinity chromatography. Disulfide bonds within the polypeptide were formed prior to removal of the affinity tag. The proinsulin cleaved from the fusion protein was then subjected to a final purification step of semipreparative reversed-phase high-performance liquid chromatography. Integrity of both the normal and mutant proinsulins was confirmed by peptide mapping and mass spectrometry. The different versions of proinsulin will be used to map those residues of the substrate used in cleavage site recognition by members of the furin/PC family of converting enzymes.

Original language	English (US)
Pages (from-to)	308-313
Number of pages	6
Journal	Protein Expression and Purification
Volume	15
Issue number	3
DOIs	https://doi.org/10.1006/prep.1998.1024
State	Published - Apr 1999
Externally published	Yes

ASJC Scopus subject areas

Biotechnology

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10.1006/prep.1998.1024

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title = "Streamlined procedure for the production of normal and altered versions of recombinant human proinsulin",

abstract = "A method for the simplified, reproducible production of both normal and altered versions of human proinsulin has been developed. A polyhistidine/proinsulin fusion protein was expressed using a prokaryotic expression system and partially purified by affinity chromatography. Disulfide bonds within the polypeptide were formed prior to removal of the affinity tag. The proinsulin cleaved from the fusion protein was then subjected to a final purification step of semipreparative reversed-phase high-performance liquid chromatography. Integrity of both the normal and mutant proinsulins was confirmed by peptide mapping and mass spectrometry. The different versions of proinsulin will be used to map those residues of the substrate used in cleavage site recognition by members of the furin/PC family of converting enzymes.",

author = "Mackin, {Robert B.}",

note = "Funding Information: The author thanks Amy Johnson for excellent technical assistance and perseverance during the course of this project. He also thanks Dr. Al Williams of Pharmacia for a number of helpful discussions, Eli Lilly and Co. for providing human proinsulin for use as a standard, and Martha Figueroa and Stacey Vondra for additional technical assistance. In addition, he thanks Drs. Y. Peng Loh and Fu-Sheng Shen (NIH) for performing the site-directed mutagenesis and DNA sequence analysis of the plasmid encoding H10D hPI. This work was funded by grants from the National Institutes of Health (DK 52085) and the State of Nebraska Cancer and Smoking-Related Disease Program. Funding for the electrospray ionization–mass spectrometer was obtained from the Nebraska EPSCoR Program.",

year = "1999",

month = apr,

doi = "10.1006/prep.1998.1024",

language = "English (US)",

volume = "15",

pages = "308--313",

journal = "Protein Expression and Purification",

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AU - Mackin, Robert B.

N1 - Funding Information: The author thanks Amy Johnson for excellent technical assistance and perseverance during the course of this project. He also thanks Dr. Al Williams of Pharmacia for a number of helpful discussions, Eli Lilly and Co. for providing human proinsulin for use as a standard, and Martha Figueroa and Stacey Vondra for additional technical assistance. In addition, he thanks Drs. Y. Peng Loh and Fu-Sheng Shen (NIH) for performing the site-directed mutagenesis and DNA sequence analysis of the plasmid encoding H10D hPI. This work was funded by grants from the National Institutes of Health (DK 52085) and the State of Nebraska Cancer and Smoking-Related Disease Program. Funding for the electrospray ionization–mass spectrometer was obtained from the Nebraska EPSCoR Program.

PY - 1999/4

Y1 - 1999/4

N2 - A method for the simplified, reproducible production of both normal and altered versions of human proinsulin has been developed. A polyhistidine/proinsulin fusion protein was expressed using a prokaryotic expression system and partially purified by affinity chromatography. Disulfide bonds within the polypeptide were formed prior to removal of the affinity tag. The proinsulin cleaved from the fusion protein was then subjected to a final purification step of semipreparative reversed-phase high-performance liquid chromatography. Integrity of both the normal and mutant proinsulins was confirmed by peptide mapping and mass spectrometry. The different versions of proinsulin will be used to map those residues of the substrate used in cleavage site recognition by members of the furin/PC family of converting enzymes.

AB - A method for the simplified, reproducible production of both normal and altered versions of human proinsulin has been developed. A polyhistidine/proinsulin fusion protein was expressed using a prokaryotic expression system and partially purified by affinity chromatography. Disulfide bonds within the polypeptide were formed prior to removal of the affinity tag. The proinsulin cleaved from the fusion protein was then subjected to a final purification step of semipreparative reversed-phase high-performance liquid chromatography. Integrity of both the normal and mutant proinsulins was confirmed by peptide mapping and mass spectrometry. The different versions of proinsulin will be used to map those residues of the substrate used in cleavage site recognition by members of the furin/PC family of converting enzymes.

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IS - 3

ER -

Streamlined procedure for the production of normal and altered versions of recombinant human proinsulin

Abstract

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