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Pak. J. Bot., 48(1): 363-370, 2016.

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  Updated: 29-02-16

 

 

MOLECULAR CHARACTERIZATION OF YEAST STRAINS ISOLATED FROM DIFFERENT SOURCES BY RESTRICTION FRAGMENT LENGTH POLYMORPHISM

 

MUHAMMAD SHAHZAD ALI AND ZAKIA LATIF*

 

Abstract: Various molecular techniques like analysis of the amplified rDNA internal transcribed spacers (ITS), intragenic spacers and total ITS region analysis by restriction fragment length polymorphism (RFLP) has been introduced for yeast identification but there are limited databases to identify yeast species on the basis of 5.8S rDNA. In this study, twenty nineyeast strains from various sources including spoiled fruits, vegetables, foodstuffs, and concentrated juices were  characterized by PCR-RFLP. PCR-RFLP has been used to characterize yeasts present in different spoiled food samples after isolation of the yeasts. By using this technique, the isolated yeast strains were characterized by direct 5.8S-ITS rDNA region amplification. RFLP analysis was applied to each of the amplification products (varied from 400bp to 800bp) detected, and  the corresponding yeast identifications were made according to each specific restriction patterns obtained after treatment with two endonucleases TaqI and HaeIII which yielded a specific banding pattern for each species. For further confirmation amplified products of eleven selected isolates were sequenced and blast on NCBI. Both RFLP and sequence analyses of the strains with accession nos. KF472163, KF472164, KF472165, KF472166, KF472167, KF472168, KF472169, KF472170, KF472171, KF472172, KF472173 gave significantly similar results. The isolates were found to belong five different yeast species including; Candida spp., Pichia spp., Kluyveromyces spp., Clavispora spp. and Hanseniaspora spp. This method provides a fast, easy, reliable and authentic way for determining yeast population present in different type of samples, as compared to traditional characterization technique

 

Key words: Yeast; RFLP; 5.8S-ITS; Candida; Pichia: Clavispora.

 


Department of Microbiology & Molecular Genetics, University of the Punjab, Quaid-e-Azam Campus, Lahore, Pakistan

*Corresponding author’s email: zakia.mmg@pu.edu.pk


   
   

 

   
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