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Purification and characterization of an exon 2-deleted human β-tropomyosin constructed by the polymerase chain reaction
- Source :
- Protein Expression and Purification. 2:188-193
- Publication Year :
- 1991
- Publisher :
- Elsevier BV, 1991.
-
Abstract
- We deleted exon 2 in human skeletal beta-tropomyosin (h beta-SK tropomyosin) using an improved adaptation of polymerase chain reaction (PCR) technology. The first PCR product was used to prime the full-length cDNA, leading to an exon 2-deleted h beta-SK tropomyosin. This new protein, des-(39-80)-tropomyosin, could then be expressed in Escherichia coli and purified to homogeneity. At the nucleotide level, the junction between exons 1 and 3 has been precisely made in the PCR product. The mutated protein was purified using high-performance liquid chromatography. Des-(39-80)-tropomyosin revealed new immunological properties but was still recognized by certain antitropomyosin antibodies. Furthermore, the structural characteristics of the mutated tropomyosin fit those of the full-length tropomyosin. This new adaptation of PCR technology appears to be suitable for every kind of mutation inside a cloned DNA molecule, and one mutation primer per mutation is sufficient.
- Subjects :
- Molecular Sequence Data
Tropomyosin
macromolecular substances
Biology
medicine.disease_cause
Polymerase Chain Reaction
law.invention
chemistry.chemical_compound
Exon
law
Complementary DNA
Escherichia coli
medicine
Humans
Cloning, Molecular
Chromatography, High Pressure Liquid
Polymerase chain reaction
Mutation
Base Sequence
DNA
Exons
musculoskeletal system
Molecular biology
Recombinant Proteins
chemistry
Biochemistry
Mutagenesis, Site-Directed
Chromosome Deletion
Primer (molecular biology)
tissues
Biotechnology
Subjects
Details
- ISSN :
- 10465928
- Volume :
- 2
- Database :
- OpenAIRE
- Journal :
- Protein Expression and Purification
- Accession number :
- edsair.doi.dedup.....767c4be0deff8f4496fbb660e7b2eb05
- Full Text :
- https://doi.org/10.1016/1046-5928(91)90070-y