The T7 concatemer junction sequence interferes with expression from a downstream T7 promoter in vivo

Bohdan Harvey; Malgorzata Korus; Emanuel Goldman

The T7 concatemer junction sequence interferes with expression from a downstream T7 promoter in vivo

Bohdan Harvey, Malgorzata Korus, Emanuel Goldman

New Jersey Medical School (NJMS), Microbiology

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

5 Scopus citations

Abstract

A recently described new signal for transcription termination in vitro by T7 RNA polymerase has now been tested in vivo. This signal, identified during transcription of the cloned human preproparathyroid hormone (PTH) gene, is also found in the phage T7 genome, at the concatemer junction (CJ). We introduced the 17-bp concatemer junction sequence at the ends of a test gene and control gene (both derived from T7 gene 9) in a T7 vector previously used to study effects of rare codons on expression. The CJ elements replaced the original vector's RNase llI processing sites, and a new T7 promoter was also introduced to drive the downstream (control) gene. We assayed for test and control gene mRNA and protein by direct labeling with [³²P]phosphate and [³⁵S]methionine. The altered vector with CJ sequences (pCTl.1) expressed the upstream test gene, but showed poor expression of the downstream control gene. No discrete T7 mRNA bands could be discerned by direct labeling with ³²P. A precursor vector with only the control gene in single copy expressed the protein much better, suggesting that the inhibition of control gene expression in pCTl.1 was a result of the upstream CJ element at the 3' end of the test gene. RT-PCR experiments were consistent with readthrough and possibly pausing at CJ. An RNA folding program predicts a highly stable secondary structure between the upstream CJ element and the control gene's translation start signals. These data support an interpretation that the CJ element is ineffective as a T7 transcription terminator in vivo in this vector, and that structure of the readthrough transcript blocks ribosome access to the downstream translation start. The readthrough transcripts are also likely to be less stable than properly terminated or processed T7 mRNA, because levels of test protein expression in pCTl.1 were reduced compared to original vector, and basal expression was negligible, while the original codon test vector shows substantial basal expression.

Original language	English (US)
Pages (from-to)	141-149
Number of pages	9
Journal	GENE EXPRESSION
Volume	8
Issue number	3
State	Published - 1999

All Science Journal Classification (ASJC) codes

Molecular Biology
Genetics

Keywords

Concatemer junction
Preproparathyroid hormone
T7 promoter

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@article{406e632935a24ecabb68f345d30f7599,

title = "The T7 concatemer junction sequence interferes with expression from a downstream T7 promoter in vivo",

abstract = "A recently described new signal for transcription termination in vitro by T7 RNA polymerase has now been tested in vivo. This signal, identified during transcription of the cloned human preproparathyroid hormone (PTH) gene, is also found in the phage T7 genome, at the concatemer junction (CJ). We introduced the 17-bp concatemer junction sequence at the ends of a test gene and control gene (both derived from T7 gene 9) in a T7 vector previously used to study effects of rare codons on expression. The CJ elements replaced the original vector's RNase llI processing sites, and a new T7 promoter was also introduced to drive the downstream (control) gene. We assayed for test and control gene mRNA and protein by direct labeling with [32P]phosphate and [35S]methionine. The altered vector with CJ sequences (pCTl.1) expressed the upstream test gene, but showed poor expression of the downstream control gene. No discrete T7 mRNA bands could be discerned by direct labeling with 32P. A precursor vector with only the control gene in single copy expressed the protein much better, suggesting that the inhibition of control gene expression in pCTl.1 was a result of the upstream CJ element at the 3' end of the test gene. RT-PCR experiments were consistent with readthrough and possibly pausing at CJ. An RNA folding program predicts a highly stable secondary structure between the upstream CJ element and the control gene's translation start signals. These data support an interpretation that the CJ element is ineffective as a T7 transcription terminator in vivo in this vector, and that structure of the readthrough transcript blocks ribosome access to the downstream translation start. The readthrough transcripts are also likely to be less stable than properly terminated or processed T7 mRNA, because levels of test protein expression in pCTl.1 were reduced compared to original vector, and basal expression was negligible, while the original codon test vector shows substantial basal expression.",

keywords = "Concatemer junction, Preproparathyroid hormone, T7 promoter",

author = "Bohdan Harvey and Malgorzata Korus and Emanuel Goldman",

year = "1999",

language = "English (US)",

volume = "8",

pages = "141--149",

journal = "Gene Expression",

issn = "1052-2166",

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TY - JOUR

T1 - The T7 concatemer junction sequence interferes with expression from a downstream T7 promoter in vivo

AU - Harvey, Bohdan

AU - Korus, Malgorzata

AU - Goldman, Emanuel

PY - 1999

Y1 - 1999

N2 - A recently described new signal for transcription termination in vitro by T7 RNA polymerase has now been tested in vivo. This signal, identified during transcription of the cloned human preproparathyroid hormone (PTH) gene, is also found in the phage T7 genome, at the concatemer junction (CJ). We introduced the 17-bp concatemer junction sequence at the ends of a test gene and control gene (both derived from T7 gene 9) in a T7 vector previously used to study effects of rare codons on expression. The CJ elements replaced the original vector's RNase llI processing sites, and a new T7 promoter was also introduced to drive the downstream (control) gene. We assayed for test and control gene mRNA and protein by direct labeling with [32P]phosphate and [35S]methionine. The altered vector with CJ sequences (pCTl.1) expressed the upstream test gene, but showed poor expression of the downstream control gene. No discrete T7 mRNA bands could be discerned by direct labeling with 32P. A precursor vector with only the control gene in single copy expressed the protein much better, suggesting that the inhibition of control gene expression in pCTl.1 was a result of the upstream CJ element at the 3' end of the test gene. RT-PCR experiments were consistent with readthrough and possibly pausing at CJ. An RNA folding program predicts a highly stable secondary structure between the upstream CJ element and the control gene's translation start signals. These data support an interpretation that the CJ element is ineffective as a T7 transcription terminator in vivo in this vector, and that structure of the readthrough transcript blocks ribosome access to the downstream translation start. The readthrough transcripts are also likely to be less stable than properly terminated or processed T7 mRNA, because levels of test protein expression in pCTl.1 were reduced compared to original vector, and basal expression was negligible, while the original codon test vector shows substantial basal expression.

AB - A recently described new signal for transcription termination in vitro by T7 RNA polymerase has now been tested in vivo. This signal, identified during transcription of the cloned human preproparathyroid hormone (PTH) gene, is also found in the phage T7 genome, at the concatemer junction (CJ). We introduced the 17-bp concatemer junction sequence at the ends of a test gene and control gene (both derived from T7 gene 9) in a T7 vector previously used to study effects of rare codons on expression. The CJ elements replaced the original vector's RNase llI processing sites, and a new T7 promoter was also introduced to drive the downstream (control) gene. We assayed for test and control gene mRNA and protein by direct labeling with [32P]phosphate and [35S]methionine. The altered vector with CJ sequences (pCTl.1) expressed the upstream test gene, but showed poor expression of the downstream control gene. No discrete T7 mRNA bands could be discerned by direct labeling with 32P. A precursor vector with only the control gene in single copy expressed the protein much better, suggesting that the inhibition of control gene expression in pCTl.1 was a result of the upstream CJ element at the 3' end of the test gene. RT-PCR experiments were consistent with readthrough and possibly pausing at CJ. An RNA folding program predicts a highly stable secondary structure between the upstream CJ element and the control gene's translation start signals. These data support an interpretation that the CJ element is ineffective as a T7 transcription terminator in vivo in this vector, and that structure of the readthrough transcript blocks ribosome access to the downstream translation start. The readthrough transcripts are also likely to be less stable than properly terminated or processed T7 mRNA, because levels of test protein expression in pCTl.1 were reduced compared to original vector, and basal expression was negligible, while the original codon test vector shows substantial basal expression.

KW - Concatemer junction

KW - Preproparathyroid hormone

KW - T7 promoter

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M3 - Article

C2 - 10634316

AN - SCOPUS:0033385013

SN - 1052-2166

VL - 8

SP - 141

EP - 149

JO - Gene Expression

JF - Gene Expression

IS - 3

ER -

The T7 concatemer junction sequence interferes with expression from a downstream T7 promoter in vivo

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