English
 
Help Privacy Policy Disclaimer
  Advanced SearchBrowse

Item

ITEM ACTIONSEXPORT
 
 
DownloadE-Mail
  Enzymatic amplification of myosin heavy-chain mRNA sequences in vitro

Harbarth, P., & Vosberg, H.-P. (1988). Enzymatic amplification of myosin heavy-chain mRNA sequences in vitro. DNA, 7(4), 297-306. doi:10.1089/dna.1988.7.297.

Item is

Files

show Files
hide Files
:
DNA_7_1988_297.pdf (Any fulltext), 6MB
 
File Permalink:
-
Name:
DNA_7_1988_297.pdf
Description:
-
OA-Status:
Visibility:
Restricted (Max Planck Institute for Medical Research, MHMF; )
MIME-Type / Checksum:
application/pdf
Technical Metadata:
Copyright Date:
-
Copyright Info:
-
License:
-

Locators

show
hide
Description:
-
OA-Status:
Description:
-
OA-Status:

Creators

show
hide
 Creators:
Harbarth, Peter1, Author           
Vosberg, Hans-Peter1, Author           
Affiliations:
1Department of Molecular Biology, Max Planck Institute for Medical Research, Max Planck Society, ou_1497702              

Content

show
hide
Free keywords: -
 Abstract: We have developed a procedure that detects the presence of mRNA coding for human beta-myosin heavy chain in small amounts of total, unfractionated RNA isolated from heart or skeletal muscle. The protocol is based on the enzymatic amplification in vitro of a selected 106-bp myosin isotype-specific subregion of this mRNA. The method, which is a modification of the so-called "polymerase chain reaction," requires two synthetic oligonucleotide primers (20-mers), reverse transcriptase, and DNA polymerase I (Klenow fragment). Two principle steps are involved: (i) the selected mRNA subregion is converted into a double-stranded cDNA, and (ii) this cDNA is amplified in 22 synthetic cycles. After gel electrophoresis and blotting the amplification product is identified by hybridization with a third oligonucleotide recognizing the region between the two primer annealing sites, and by restriction mapping. Only mRNA from muscle tissue promoted formation of the amplified 106-bp fragment. We estimate that less than 30,000 beta-myosin heavy-chain mRNA molecules are sufficient to produce a signal. The procedure is fast, specific, and very sensitive. It may be used in muscle gene expression studies with small numbers of cells or even in single muscle fibers.

Details

show
hide
Language(s): eng - English
 Dates: 1987-10-271987-07-201988-05
 Publication Status: Issued
 Pages: 10
 Publishing info: -
 Table of Contents: -
 Rev. Type: Peer
 Degree: -

Event

show

Legal Case

show

Project information

show

Source 1

show
hide
Title: DNA
  Other : DNA
Source Genre: Journal
 Creator(s):
Affiliations:
Publ. Info: New York : Mary Ann Liebert
Pages: - Volume / Issue: 7 (4) Sequence Number: - Start / End Page: 297 - 306 Identifier: ISSN: 0198-0238
CoNE: https://pure.mpg.de/cone/journals/resource/954925275481