Human protein disulfide isomerase functionally complements a dsbA mutation and enhances the yield of pectate lyase C in Escherichia coli

D P Humphreys; N Weir; A Mountain; P A Lund

Human protein disulfide isomerase functionally complements a dsbA mutation and enhances the yield of pectate lyase C in Escherichia coli

D P Humphreys, N Weir, A Mountain, P A Lund

Biosciences

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

49 Citations (Scopus)

Abstract

Human PDI was expressed to the Escherichia coli periplasm, by using a plasmid encoded ompA-PDI fusion under the control of the trp promoter. Periplasmic extracts were shown to contain active PDI using the scrambled ribonuclease assay. PDI activity was also demonstrated by complementation of two phenotypes associated with a dsbA mutation. Alkaline phosphatase activity, which is reduced in dsbA cells, was restored to wild type levels by PDI. PelC, a pectate lyase from Erwinia carotovora, was shown to be DsbA dependent in E. coli. PDI was able to restore its activity to that seen in wild type cells. Increased expression of PDI was found to increase the yield of active PelC above that seen in wild type cells. PDI also enhanced the yield of PelC in DsbA- cells but only in the presence of exogenous oxidized glutathione. PDI is thus able to functionally substitute for DsbA in the folding of disulfide-bonded proteins in the bacterial periplasm and to enhance the yield of highly expressed protein when the ability of the E. coli periplasm to fold protein may be saturated. However, our results suggest that the activities of DsbA and PDI in vivo may be different.

Original language	English
Pages (from-to)	28210-5
Number of pages	6
Journal	Journal of Biological Chemistry
Volume	270
Issue number	47
Publication status	Published - 24 Nov 1995

Keywords

Protein Disulfide-Isomerases
Genes, Bacterial
Recombinant Proteins
Humans
Isomerases
Polysaccharide-Lyases
Plasmids
Cloning, Molecular
Mutagenesis, Site-Directed
Polymerase Chain Reaction
Base Sequence
Blotting, Western
Kinetics
Restriction Mapping
DNA Primers
Escherichia coli
Genetic Complementation Test
Isoenzymes
Molecular Sequence Data
Erwinia

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title = "Human protein disulfide isomerase functionally complements a dsbA mutation and enhances the yield of pectate lyase C in Escherichia coli",

abstract = "Human PDI was expressed to the Escherichia coli periplasm, by using a plasmid encoded ompA-PDI fusion under the control of the trp promoter. Periplasmic extracts were shown to contain active PDI using the scrambled ribonuclease assay. PDI activity was also demonstrated by complementation of two phenotypes associated with a dsbA mutation. Alkaline phosphatase activity, which is reduced in dsbA cells, was restored to wild type levels by PDI. PelC, a pectate lyase from Erwinia carotovora, was shown to be DsbA dependent in E. coli. PDI was able to restore its activity to that seen in wild type cells. Increased expression of PDI was found to increase the yield of active PelC above that seen in wild type cells. PDI also enhanced the yield of PelC in DsbA- cells but only in the presence of exogenous oxidized glutathione. PDI is thus able to functionally substitute for DsbA in the folding of disulfide-bonded proteins in the bacterial periplasm and to enhance the yield of highly expressed protein when the ability of the E. coli periplasm to fold protein may be saturated. However, our results suggest that the activities of DsbA and PDI in vivo may be different.",

keywords = "Protein Disulfide-Isomerases, Genes, Bacterial, Recombinant Proteins, Humans, Isomerases, Polysaccharide-Lyases, Plasmids, Cloning, Molecular, Mutagenesis, Site-Directed, Polymerase Chain Reaction, Base Sequence, Blotting, Western, Kinetics, Restriction Mapping, DNA Primers, Escherichia coli, Genetic Complementation Test, Isoenzymes, Molecular Sequence Data, Erwinia",

author = "Humphreys, {D P} and N Weir and A Mountain and Lund, {P A}",

year = "1995",

month = nov,

day = "24",

language = "English",

volume = "270",

pages = "28210--5",

journal = "Journal of Biological Chemistry",

issn = "0021-9258",

publisher = "American Society for Biochemistry and Molecular Biology",

number = "47",

}

TY - JOUR

T1 - Human protein disulfide isomerase functionally complements a dsbA mutation and enhances the yield of pectate lyase C in Escherichia coli

AU - Humphreys, D P

AU - Weir, N

AU - Mountain, A

AU - Lund, P A

PY - 1995/11/24

Y1 - 1995/11/24

N2 - Human PDI was expressed to the Escherichia coli periplasm, by using a plasmid encoded ompA-PDI fusion under the control of the trp promoter. Periplasmic extracts were shown to contain active PDI using the scrambled ribonuclease assay. PDI activity was also demonstrated by complementation of two phenotypes associated with a dsbA mutation. Alkaline phosphatase activity, which is reduced in dsbA cells, was restored to wild type levels by PDI. PelC, a pectate lyase from Erwinia carotovora, was shown to be DsbA dependent in E. coli. PDI was able to restore its activity to that seen in wild type cells. Increased expression of PDI was found to increase the yield of active PelC above that seen in wild type cells. PDI also enhanced the yield of PelC in DsbA- cells but only in the presence of exogenous oxidized glutathione. PDI is thus able to functionally substitute for DsbA in the folding of disulfide-bonded proteins in the bacterial periplasm and to enhance the yield of highly expressed protein when the ability of the E. coli periplasm to fold protein may be saturated. However, our results suggest that the activities of DsbA and PDI in vivo may be different.

AB - Human PDI was expressed to the Escherichia coli periplasm, by using a plasmid encoded ompA-PDI fusion under the control of the trp promoter. Periplasmic extracts were shown to contain active PDI using the scrambled ribonuclease assay. PDI activity was also demonstrated by complementation of two phenotypes associated with a dsbA mutation. Alkaline phosphatase activity, which is reduced in dsbA cells, was restored to wild type levels by PDI. PelC, a pectate lyase from Erwinia carotovora, was shown to be DsbA dependent in E. coli. PDI was able to restore its activity to that seen in wild type cells. Increased expression of PDI was found to increase the yield of active PelC above that seen in wild type cells. PDI also enhanced the yield of PelC in DsbA- cells but only in the presence of exogenous oxidized glutathione. PDI is thus able to functionally substitute for DsbA in the folding of disulfide-bonded proteins in the bacterial periplasm and to enhance the yield of highly expressed protein when the ability of the E. coli periplasm to fold protein may be saturated. However, our results suggest that the activities of DsbA and PDI in vivo may be different.

KW - Protein Disulfide-Isomerases

KW - Genes, Bacterial

KW - Recombinant Proteins

KW - Humans

KW - Isomerases

KW - Polysaccharide-Lyases

KW - Plasmids

KW - Cloning, Molecular

KW - Mutagenesis, Site-Directed

KW - Polymerase Chain Reaction

KW - Base Sequence

KW - Blotting, Western

KW - Kinetics

KW - Restriction Mapping

KW - DNA Primers

KW - Escherichia coli

KW - Genetic Complementation Test

KW - Isoenzymes

KW - Molecular Sequence Data

KW - Erwinia

M3 - Article

C2 - 7499315

SN - 0021-9258

VL - 270

SP - 28210

EP - 28215

JO - Journal of Biological Chemistry

JF - Journal of Biological Chemistry

IS - 47

ER -

Human protein disulfide isomerase functionally complements a dsbA mutation and enhances the yield of pectate lyase C in Escherichia coli

Abstract

Keywords

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