Chia Nan University of Pharmacy & Science Institutional Repository:Item 310902800/22797
English  |  正體中文  |  简体中文  |  Items with full text/Total items : 18034/20233 (89%)
Visitors : 23727674      Online Users : 737
RC Version 7.0 © Powered By DSPACE, MIT. Enhanced by NTU Library IR team.
Scope Tips:
  • please add "double quotation mark" for query phrases to get precise results
  • please goto advance search for comprehansive author search
    •  Adv. Search
    HomeLoginUploadHelpAboutAdminister Goto mobile version
    CNU IR > Chna Nan Annual Bulletin > Vol.35 (2009) >  Item 310902800/22797


    Please use this identifier to cite or link to this item: https://ir.cnu.edu.tw/handle/310902800/22797


    Title: Identification of acetic acid bacteria isolates from home made fermentation liquids by PCR
    應用聚合醃鏈反應(PCR)技術鑑定分離自傳統家庭釀造液之醋酸菌
    Authors: Shu-Jen Wang
    Min-Hsiu Chang
    Chen-Kai Chang
    Jiau-Hua Chen
    Contributors: 食品科技系
    Keywords: acetic acid bacteria
    adh III sequence
    PCR
    Acetobacter sp.
    醋酸菌
    酒精去氫醣Ⅲ序列
    聚合酶鏈反應
    醋酸菌屬
    Date: 2009
    Issue Date: 2010-09-10 09:09:05 (UTC+8)
    Abstract: In this study, polymerase chain reaction primers based on adh Ill sequence (GenBank accession no. AB264314) were designed for identification ofAcetobacter strains and acetic acid bacteria (MB) isolates. This primer set termed 4DH 187/ADH 500ns successfitlly usedw identification of41 MB strains of 79 isolates rectly kom homemade vinegar fermentation. Furthermore, the acetate oxidation ability was sed for analysis ofacetate oxidation ability. Theesults showed that the AAB305 strain could roduce higher acetate content than ither AAB isolates in Yeast Glucose Mannitol/ Mg2 (YGN/UMg2.) nedium supplemented with 7% ethanol and could be used for industrial negar production. In addition, these isolates with high .cetate oxidation ability were identified as Acetobacter sp. by the equencing ofthe 16S rDNA PCR amplification products.
    本研究根據醋酸菌之 adh III序列( GenBank access ion no. AB264314 ),發展特異性PCR引子,ADH187/ADH 500,此PCR引子成功的應用於醋酸菌菌株及非醋酸菌菌株之檢測。將此PCR引子應用於家庭自釀醋中離之79株疑似醋酸菌株之檢測,其中41株經KR引子初步確認為醋酸菌。以醋酸產生能力分析篩選出29株,至一步分析29株分離之醋酸菌之醋酸產量及酒精耐受度,發現分離株AAB305 士含7% ( v/v )乙醇之Yeastlucose Mannitol/ Mg2+ YGM/Mg為) medi um中比其他分離株產生更高醋酸量,將來可進一步應用於工業上醋酸之生產。侍醋酸產量高之分離株經16S「現1A序列分析確認皆為Ac今tobacter spp.。由結果顯亓,此PCR方法與165 rDNA序列分析結果符合,將PCR方法應用於醋酸菌的篩選可節省大量人力及物力。
    Relation: 嘉南學報(科技類) 35:p.199-210
    Appears in Collections:[Chna Nan Annual Bulletin] Vol.35 (2009)
    [Dept. of Food Science & Technology] Periodical Articles

    Files in This Item:

    File Description SizeFormat
    v35_199_210.pdf10553KbAdobe PDF666View/Open


    All items in CNU IR are protected by copyright, with all rights reserved.

    DSpace Software Copyright © 2002-2004  MIT &  Hewlett-Packard  /   Enhanced by   NTU Library IR team Copyright ©   - Feedback