High-level production of hepatitis B viral X protein in Escherichia coli using gene II promoter of bacteriophage M13

Mong Liang Chen; Yan-Hwa Wu Lee; Szecheng J. Lo

doi:10.1016/0378-1119(88)90568-9

High-level production of hepatitis B viral X protein in Escherichia coli using gene II promoter of bacteriophage M13

Mong Liang Chen, Yan-Hwa Wu Lee, Szecheng J. Lo^*

^*Corresponding author for this work

Department of Biological Science and Technology

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

8 Scopus citations

Abstract

Region X is one of the four open reading frames (ORFs) of hepatitits B virus (HBV) and encodes a polypeptide of 154 amino acids (aa). A 584-bp BamHI-BglII fragment of the HBV DNA containing the major part of ORF X which encodes 145 aawas inserted into the BglII site within the gene II of bacteriophage M13. The insertion resulted m an in-phase gene II-X fused protein of 174 aa under the control of the gene II promoter. Cells harboring plasmids (pMLαX.59 and pMLX.12d) derived from the above construct overproduced the 19-kDa fused protein in Escherichia coli at a level of 10%-20% of total cellular protein. The fused protein was recognized by the anti-X antibodies. This is the first demonstration of using gene II promoter of M13 to express a foreign gene efficiently.

Original language	English
Pages (from-to)	315-321
Number of pages	7
Journal	Gene
Volume	62
Issue number	2
DOIs	https://doi.org/10.1016/0378-1119(88)90568-9
State	Published - 29 Feb 1988

Keywords

Recombinant DNA
anti-X antibody
expression vector
fusion protein
immunoblot

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10.1016/0378-1119(88)90568-9

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title = "High-level production of hepatitis B viral X protein in Escherichia coli using gene II promoter of bacteriophage M13",

abstract = "Region X is one of the four open reading frames (ORFs) of hepatitits B virus (HBV) and encodes a polypeptide of 154 amino acids (aa). A 584-bp BamHI-BglII fragment of the HBV DNA containing the major part of ORF X which encodes 145 aawas inserted into the BglII site within the gene II of bacteriophage M13. The insertion resulted m an in-phase gene II-X fused protein of 174 aa under the control of the gene II promoter. Cells harboring plasmids (pMLαX.59 and pMLX.12d) derived from the above construct overproduced the 19-kDa fused protein in Escherichia coli at a level of 10%-20% of total cellular protein. The fused protein was recognized by the anti-X antibodies. This is the first demonstration of using gene II promoter of M13 to express a foreign gene efficiently.",

keywords = "Recombinant DNA, anti-X antibody, expression vector, fusion protein, immunoblot",

author = "Chen, {Mong Liang} and {Wu Lee}, Yan-Hwa and Lo, {Szecheng J.}",

year = "1988",

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doi = "10.1016/0378-1119(88)90568-9",

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T1 - High-level production of hepatitis B viral X protein in Escherichia coli using gene II promoter of bacteriophage M13

AU - Chen, Mong Liang

AU - Wu Lee, Yan-Hwa

AU - Lo, Szecheng J.

PY - 1988/2/29

Y1 - 1988/2/29

N2 - Region X is one of the four open reading frames (ORFs) of hepatitits B virus (HBV) and encodes a polypeptide of 154 amino acids (aa). A 584-bp BamHI-BglII fragment of the HBV DNA containing the major part of ORF X which encodes 145 aawas inserted into the BglII site within the gene II of bacteriophage M13. The insertion resulted m an in-phase gene II-X fused protein of 174 aa under the control of the gene II promoter. Cells harboring plasmids (pMLαX.59 and pMLX.12d) derived from the above construct overproduced the 19-kDa fused protein in Escherichia coli at a level of 10%-20% of total cellular protein. The fused protein was recognized by the anti-X antibodies. This is the first demonstration of using gene II promoter of M13 to express a foreign gene efficiently.

AB - Region X is one of the four open reading frames (ORFs) of hepatitits B virus (HBV) and encodes a polypeptide of 154 amino acids (aa). A 584-bp BamHI-BglII fragment of the HBV DNA containing the major part of ORF X which encodes 145 aawas inserted into the BglII site within the gene II of bacteriophage M13. The insertion resulted m an in-phase gene II-X fused protein of 174 aa under the control of the gene II promoter. Cells harboring plasmids (pMLαX.59 and pMLX.12d) derived from the above construct overproduced the 19-kDa fused protein in Escherichia coli at a level of 10%-20% of total cellular protein. The fused protein was recognized by the anti-X antibodies. This is the first demonstration of using gene II promoter of M13 to express a foreign gene efficiently.

KW - Recombinant DNA

KW - anti-X antibody

KW - expression vector

KW - fusion protein

KW - immunoblot

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DO - 10.1016/0378-1119(88)90568-9

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AN - SCOPUS:0023855011

SN - 0378-1119

VL - 62

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EP - 321

JO - Gene

JF - Gene

IS - 2

ER -

High-level production of hepatitis B viral X protein in Escherichia coli using gene II promoter of bacteriophage M13

Abstract

Keywords

UN SDGs

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