In situ reverse transcription-PCR for monitoring gene expression in individual Methanosarcina mazei S-6 cells.

M Lange; Tim Tolker-Nielsen; S Molin; B K Ahring

In situ reverse transcription-PCR for monitoring gene expression in individual Methanosarcina mazei S-6 cells.

M Lange, Tim Tolker-Nielsen, S Molin, B K Ahring

17 Citations (Scopus)

Abstract

An in situ reverse transcription-PCR protocol for detecting specific mRNA in Methanosarcina mazei S-6 is described. This method allowed us to detect heat shock-induced increases in the intracellular levels of the transcript of the universal stress gene dnaK. The cell walls of paraformaldehyde-fixed cells were permeabilized by a thermal cycling procedure or by lysozyme treatment, and the cellular DNA was removed with DNase. The cells were subjected to a seminested reverse transcription-PCR protocol in which a digoxigenin-labeled primer was used. Detection of the reporter molecule was based on the 2-hydroxy-3-naphtoic acid-2'-phenylanilide phosphate-Fast Red detection system and binding of anti-digoxigenin-alkaline phosphatase conjugate. Fluorescence in permeabilized cells increased after a heat shock compared to fluorescence in non-heat-shocked cells, and the increase corresponded to an increase in the level of the dnaK transcript.

Original language	English
Journal	Applied and Environmental Microbiology
Volume	66
Issue number	5
Pages (from-to)	1796-800
Number of pages	4
ISSN	0099-2240
Publication status	Published - 2000
Externally published	Yes

Cite this

@article{e4a5add0bd4111dd8e02000ea68e967b,

title = "In situ reverse transcription-PCR for monitoring gene expression in individual Methanosarcina mazei S-6 cells.",

abstract = "An in situ reverse transcription-PCR protocol for detecting specific mRNA in Methanosarcina mazei S-6 is described. This method allowed us to detect heat shock-induced increases in the intracellular levels of the transcript of the universal stress gene dnaK. The cell walls of paraformaldehyde-fixed cells were permeabilized by a thermal cycling procedure or by lysozyme treatment, and the cellular DNA was removed with DNase. The cells were subjected to a seminested reverse transcription-PCR protocol in which a digoxigenin-labeled primer was used. Detection of the reporter molecule was based on the 2-hydroxy-3-naphtoic acid-2'-phenylanilide phosphate-Fast Red detection system and binding of anti-digoxigenin-alkaline phosphatase conjugate. Fluorescence in permeabilized cells increased after a heat shock compared to fluorescence in non-heat-shocked cells, and the increase corresponded to an increase in the level of the dnaK transcript.",

author = "M Lange and Tim Tolker-Nielsen and S Molin and Ahring, {B K}",

note = "Keywords: Cell Wall; DNA Primers; Digoxigenin; Escherichia coli Proteins; HSP70 Heat-Shock Proteins; Indicators and Reagents; Methanosarcina; Molecular Chaperones; Muramidase; RNA, Archaeal; RNA, Messenger; Reverse Transcriptase Polymerase Chain Reaction; Transcription, Genetic",

year = "2000",

language = "English",

volume = "66",

pages = "1796--800",

journal = "Applied and Environmental Microbiology",

issn = "0099-2240",

publisher = "American Society for Microbiology",

number = "5",

}

TY - JOUR

T1 - In situ reverse transcription-PCR for monitoring gene expression in individual Methanosarcina mazei S-6 cells.

AU - Lange, M

AU - Tolker-Nielsen, Tim

AU - Molin, S

AU - Ahring, B K

N1 - Keywords: Cell Wall; DNA Primers; Digoxigenin; Escherichia coli Proteins; HSP70 Heat-Shock Proteins; Indicators and Reagents; Methanosarcina; Molecular Chaperones; Muramidase; RNA, Archaeal; RNA, Messenger; Reverse Transcriptase Polymerase Chain Reaction; Transcription, Genetic

PY - 2000

Y1 - 2000

N2 - An in situ reverse transcription-PCR protocol for detecting specific mRNA in Methanosarcina mazei S-6 is described. This method allowed us to detect heat shock-induced increases in the intracellular levels of the transcript of the universal stress gene dnaK. The cell walls of paraformaldehyde-fixed cells were permeabilized by a thermal cycling procedure or by lysozyme treatment, and the cellular DNA was removed with DNase. The cells were subjected to a seminested reverse transcription-PCR protocol in which a digoxigenin-labeled primer was used. Detection of the reporter molecule was based on the 2-hydroxy-3-naphtoic acid-2'-phenylanilide phosphate-Fast Red detection system and binding of anti-digoxigenin-alkaline phosphatase conjugate. Fluorescence in permeabilized cells increased after a heat shock compared to fluorescence in non-heat-shocked cells, and the increase corresponded to an increase in the level of the dnaK transcript.

AB - An in situ reverse transcription-PCR protocol for detecting specific mRNA in Methanosarcina mazei S-6 is described. This method allowed us to detect heat shock-induced increases in the intracellular levels of the transcript of the universal stress gene dnaK. The cell walls of paraformaldehyde-fixed cells were permeabilized by a thermal cycling procedure or by lysozyme treatment, and the cellular DNA was removed with DNase. The cells were subjected to a seminested reverse transcription-PCR protocol in which a digoxigenin-labeled primer was used. Detection of the reporter molecule was based on the 2-hydroxy-3-naphtoic acid-2'-phenylanilide phosphate-Fast Red detection system and binding of anti-digoxigenin-alkaline phosphatase conjugate. Fluorescence in permeabilized cells increased after a heat shock compared to fluorescence in non-heat-shocked cells, and the increase corresponded to an increase in the level of the dnaK transcript.

M3 - Journal article

C2 - 10788341

SN - 0099-2240

VL - 66

SP - 1796

EP - 1800

JO - Applied and Environmental Microbiology

JF - Applied and Environmental Microbiology

IS - 5

ER -

In situ reverse transcription-PCR for monitoring gene expression in individual Methanosarcina mazei S-6 cells.

Abstract

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