宁波大学学报(理工版)
寧波大學學報(理工版)
저파대학학보(리공판)
JOURNAL OF NINGBO UNIVERSITY(NSEE)
2013年
3期
11-16
,共6页
周海波%徐继林%朱鹏%严小军
週海波%徐繼林%硃鵬%嚴小軍
주해파%서계림%주붕%엄소군
滩涂贝类%饵料微藻%CTAB%18S rDNA%特异性引物
灘塗貝類%餌料微藻%CTAB%18S rDNA%特異性引物
탄도패류%이료미조%CTAB%18S rDNA%특이성인물
intertidal shellfish%diet microalgae%CTAB%18S rDNA%specific primes
用改良CTAB法提取我国沿海东南部滩涂贝类常见的4种饵料微藻的基因组DNA,结果发现提取的DNA产率高、完整性好,认为是一种简便而高效的微藻基因组DNA提取方法.对其18S rRNA 基因(18S rDNA)进行克隆与测序,并利用序列比对软件 MEGA 5.0对各微藻的18S rDNA序列进行两两比对,设计出了能够用于快速区分此4对饵料微藻的特异性PCR引物(Cha.F/Cha.R、Iso.F/Iso.R、Pla.F/Pla.R及Nan.F/Nan.R). PCR扩增验证实验结果显示,4对引物均具有很强的特异性,无交叉扩增现象.扩增片段大小范围为100~200 bp,满足实时荧光定量PCR的实验要求,在检测滩涂贝类对此4种饵料微藻的摄食选择性研究方面具有重要意义.
用改良CTAB法提取我國沿海東南部灘塗貝類常見的4種餌料微藻的基因組DNA,結果髮現提取的DNA產率高、完整性好,認為是一種簡便而高效的微藻基因組DNA提取方法.對其18S rRNA 基因(18S rDNA)進行剋隆與測序,併利用序列比對軟件 MEGA 5.0對各微藻的18S rDNA序列進行兩兩比對,設計齣瞭能夠用于快速區分此4對餌料微藻的特異性PCR引物(Cha.F/Cha.R、Iso.F/Iso.R、Pla.F/Pla.R及Nan.F/Nan.R). PCR擴增驗證實驗結果顯示,4對引物均具有很彊的特異性,無交扠擴增現象.擴增片段大小範圍為100~200 bp,滿足實時熒光定量PCR的實驗要求,在檢測灘塗貝類對此4種餌料微藻的攝食選擇性研究方麵具有重要意義.
용개량CTAB법제취아국연해동남부탄도패류상견적4충이료미조적기인조DNA,결과발현제취적DNA산솔고、완정성호,인위시일충간편이고효적미조기인조DNA제취방법.대기18S rRNA 기인(18S rDNA)진행극륭여측서,병이용서렬비대연건 MEGA 5.0대각미조적18S rDNA서렬진행량량비대,설계출료능구용우쾌속구분차4대이료미조적특이성PCR인물(Cha.F/Cha.R、Iso.F/Iso.R、Pla.F/Pla.R급Nan.F/Nan.R). PCR확증험증실험결과현시,4대인물균구유흔강적특이성,무교차확증현상.확증편단대소범위위100~200 bp,만족실시형광정량PCR적실험요구,재검측탄도패류대차4충이료미조적섭식선택성연구방면구유중요의의.
A modified CTAB method is used to extract genomic DNA from four common diet microalgae of intertidal shellfish found in southeastern coast of China, The results show that this method is very suitable for extraction of high quality and productive genomic DNA from microalgae, By cloning and sequencing of 18S rRNA gene from the four diet microalgae, their sequences are compared with each other using the software MEGA5.0, Four pairs of specific primers which can be used to quickly distinguish the microalgae in samples are designed with the help of Primer 5.0. They are named Cha.F/Cha.R, Iso.F/Iso.R, Pla.F/Pla.R and Nan.F/Nan.R. Verification tests through the PCR amplification indicate that four pairs of the primers are highly distinctive and no cross amplification phenomenon is noted. The size of these amplified fragments ranges from 100 bp to 200 bp, which meets the experimental requirements of the Real-time fluorescent quantitative PCR (qPCR). These specific primers will be of great help for the study on feeding selectivity for the diet microalgae of juvenile intertidal shellfish in China.
