云南植物研究
雲南植物研究
운남식물연구
ACTA BOTANICA YUNNANICA
2008年
3期
345-350
,共6页
郭会芳%阚显照%张韧%陈鸿珊
郭會芳%闞顯照%張韌%陳鴻珊
곽회방%감현조%장인%진홍산
鼠尾草属%ITS基因%rpl16基因%trnL-trnF基因
鼠尾草屬%ITS基因%rpl16基因%trnL-trnF基因
서미초속%ITS기인%rpl16기인%trnL-trnF기인
Salvia%ITS%rpl16%trnL-trnF
为从鼠尾草属植物中鉴别丹参品种,采用基因测序方法,用核糖体核酸内转录间隔区基因(nrDNA ITS),编码核蛋白体大亚基多肽L16的基因(rpl16)及叶绿体DNA上包含trnL以及trnL和trnF间隔区的区域基因(trnL-trnF)的序列,检测六种鼠尾草属新鲜植物.由于nrDNA ITS和rpl16突变率较高,可以做为6种鼠尾草的基源鉴定标记,依此设计了两对特异引物,从6种鼠尾草中鉴定出丹参(Salvia miltiorrhiza)和云南鼠尾草(S.yunnanensis).但trnL-trnF突变率太低,未能用于鉴别.商品干燥中药材因加工和储藏的方式致使DNA降解严重,基因测序法难于应用.
為從鼠尾草屬植物中鑒彆丹參品種,採用基因測序方法,用覈糖體覈痠內轉錄間隔區基因(nrDNA ITS),編碼覈蛋白體大亞基多肽L16的基因(rpl16)及葉綠體DNA上包含trnL以及trnL和trnF間隔區的區域基因(trnL-trnF)的序列,檢測六種鼠尾草屬新鮮植物.由于nrDNA ITS和rpl16突變率較高,可以做為6種鼠尾草的基源鑒定標記,依此設計瞭兩對特異引物,從6種鼠尾草中鑒定齣丹參(Salvia miltiorrhiza)和雲南鼠尾草(S.yunnanensis).但trnL-trnF突變率太低,未能用于鑒彆.商品榦燥中藥材因加工和儲藏的方式緻使DNA降解嚴重,基因測序法難于應用.
위종서미초속식물중감별단삼품충,채용기인측서방법,용핵당체핵산내전록간격구기인(nrDNA ITS),편마핵단백체대아기다태L16적기인(rpl16)급협록체DNA상포함trnL이급trnL화trnF간격구적구역기인(trnL-trnF)적서렬,검측륙충서미초속신선식물.유우nrDNA ITS화rpl16돌변솔교고,가이주위6충서미초적기원감정표기,의차설계료량대특이인물,종6충서미초중감정출단삼(Salvia miltiorrhiza)화운남서미초(S.yunnanensis).단trnL-trnF돌변솔태저,미능용우감별.상품간조중약재인가공화저장적방식치사DNA강해엄중,기인측서법난우응용.
Three DNA regions were sequenced for testing six fresh plant samples of Salvia species. These three DNA regions were nrDNA ITS (nuclear ribosomal DNA internal transcribed spacer), chloroplast rpl16 (the gene encoding ribosomal protein L16), and trnL-trnF (the cpDNA region comprising the trnL and the intergenic spacer between trnL and trnF). The results showed that the nrDNA ITS and rpl16 genes could provide novel information for origin identification of Salvia species. Due to their higher mutation rates of these 2 gene markers, Salvia species-specific primers were designed and S.miltiorrhiza and S.yunnanensis were identified. The trnL-trnF gene expressed low mutation rate, it could not identify the species. Since the damage of DNA by the pretreatments of the dry roots of Chinese herbs, it is hard to apply the molecular markers to commercial samples for identification.