A non-radioactive protein truncation test for the sensitive detection of all 
stop and frameshift mutations

Kahmann, Sabine; Herter, Peter; Kuhnen, Cornelius; Müller, Klaus-Michael; Muhr, Gert; Martin, Dirk; Soddemann, Matthias; Müller, Oliver

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A non-radioactive protein truncation test for the sensitive detection of all stop and frameshift mutations

Kahmann, S., Herter, P., Kuhnen, C., Müller, K.-M., Muhr, G., Martin, D., et al. (2002). A non-radioactive protein truncation test for the sensitive detection of all stop and frameshift mutations. Human Mutation, 19(2): 1, pp. 165-172. Retrieved from http://www3.interscience.wiley.com/cgi-bin/fulltext?ID=89012847&PLACEBO=IE.pdf.

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Datensatz-Permalink: https://hdl.handle.net/11858/00-001M-0000-0014-0F1B-A Versions-Permalink: https://hdl.handle.net/11858/00-001M-0000-0014-0F1C-8

Genre: Zeitschriftenartikel

Alternativer Titel : Hum. Mutat.

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Urheber:
Kahmann, Sabine¹, Autor
Herter, Peter¹, Autor
Kuhnen, Cornelius, Autor
Müller, Klaus-Michael, Autor
Muhr, Gert, Autor
Martin, Dirk, Autor
Soddemann, Matthias, Autor
Müller, Oliver², Autor

Affiliations:
1Max Planck Institute of Molecular Physiology, Max Planck Society, ou_1753286
2Sonstige Wissenschaftliche Organisationseinheiten, Max Planck Institute of Molecular Physiology, Max Planck Society, ou_1753294

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Schlagwörter: adenomatous polyposis coli; APC; hybrid capture; in vitro synthesis protein assay; IVSP; mutation detection; protein truncation test; PTT; tumor suppressor

Zusammenfassung: A new method for mutation detection is described, which is a technical advancement of the protein truncation test. The new technique is non-radioactive and highly sensitive for detection of virtually all sequence mutations, which lead to a stop signal or to the shift of the translation frame. The method includes four steps: 1) capture of the interesting sequence copies out of the sample by binding to an immobilized complementary sequence, 2) PCR amplification of the gene fragment to be analyzed with primers coding both for amino. and carboxy-terminal tags, 3) in vitro transcription and translation, and 4) analysis of the translation products by Western blot. As an evaluation of the new method, we detected mutated gene copies at a dilution of 1 to 40 compared to the non,mutated gene. Using the method, we were able to detect a mutation in the adenomatous polyposis coli tumor suppressor gene (APC) in a stool sample of a colorectal cancer patient. This mutation could not be detected by direct sequencing of the amplified APC gene fragme