Stefanov, Anguel Neykov (2006) Bulked segregant analysis as a new tool for identification and cloning of genes in Chlamydomonas reinhardtii. Identification of TBC1. Masters thesis, Concordia University.
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Abstract
Although Chlamydomonas reinhardtii is a widely used model organism for studies of a variety of cell biological processes, the identification and cloning of genes known by mutations is still arduous. Current methods are inefficient for many of the existing mutations as their mutant alleles can either spontaneously revert or produce no selectable phenotype. With the sequencing and the annotation of the C. reinhardtii nuclear genome and mapping of available molecular markers, positional cloning is now possible. This thesis explored the application of bulked segregant analysis (BSA) with two types of molecular markers, amplified fragment length polymorphisms and single nucleotide polymorphisms, in order to identify and characterize the nuclear TBC1 gene and its predicted product. TBC1 was previously shown to functionally interact with specific regions and structures in the 5' untranslated region of chloroplast psbC mRNA to promote its translation and the synthesis of its product, the CP43 subunit polypeptide of PSII. Using BSA, TBC1 was mapped to an 8 map-unit region of Linkage Group VI. Complementation analysis narrowed down its position to a 41 kb region. Analyses of predicted genes in the region identified an exonuclease II orthologue as the best candidate for being TBC1
Divisions: | Concordia University > Faculty of Arts and Science > Biology |
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Item Type: | Thesis (Masters) |
Authors: | Stefanov, Anguel Neykov |
Pagination: | xi, 180 leaves : ill. ; 29 cm. |
Institution: | Concordia University |
Degree Name: | M. Sc. |
Program: | Biology |
Date: | 2006 |
Thesis Supervisor(s): | Zerges, William |
Identification Number: | LE 3 C66B56M 2006 S84 |
ID Code: | 9009 |
Deposited By: | Concordia University Library |
Deposited On: | 18 Aug 2011 18:42 |
Last Modified: | 13 Jul 2020 20:05 |
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