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產(chǎn)品名稱:pTCK303

貨號(hào) 規(guī)格 價(jià)格 訂購(gòu)數(shù)量 是否現(xiàn)貨
ZK916 1μg(20μl,50ng/μl) 870 - + 有貨

基本信息

啟動(dòng)子:

Ubi,35s

復(fù)制子:

pUC

終止子:

NOS

質(zhì)粒分類:

植物系列,RNAi載體

原核抗性:

Kan

真核抗性:

Hyg

克隆菌株:

DH5a

培養(yǎng)條件:

37度

表達(dá)宿主:

植物細(xì)胞


質(zhì)粒屬性

質(zhì)粒宿主:

植物

質(zhì)粒用途:

基因沉默

片段類型:

shRNA

片段物種:


原核抗性:

Kan

真核抗性:

Hyg

熒光標(biāo)記:



質(zhì)粒簡(jiǎn)介

RNA interferences (RNAi) has proven to be an effective strategy to knock out homologous genes in a wide range of species. Based on its principle, a new generation of vectors containing an inverted target sequence separated by an intron as a loop, developing simplifications to the procedure of RNAi construction are required to improve the efficiency of gene inactivation techniques. Here, a novel polymerase chain reaction (PCR)—based RNAi vector pTCK303 with a maize ubiquitin promoter, 2 specific multiple enzyme sites, and a rice intron was constructed for monocot gene silencing. With this vector, only 1 PCR product amplified by a single pair of primers and 2 ligation reactions were needed to create an RNAi construct, which shortened the time span before being transformed into the plant. To test the efficiency of vector pTCK303, a rice geneOsGAS1 was used, and its RNAi construct was introduced into rice calli. Southern blot analysis of the transgenic rice confirmed the presence of theOsGAS1 RNAi structure. The decrease inOsGAS1 level in the transgenic rice was detected by Northern blot probed with anOsGAS1-specific sequence. Moreover, the rate of inhibition of the RNA expression level in RNAi transgenic rice was approximately 85% according to our real-time PCR. Therefore, the RNAi vector pTCK303 based on the homology-dependent gene-silencing mechanisms facilitated the inhibition of endogenous genes in a monocot and was proven to be a practical and efficient platform for silencing a rice gene.


質(zhì)粒圖譜


質(zhì)粒序列

質(zhì)粒序列請(qǐng)下載:ZK916pTCK303-Stuffer植物干擾質(zhì)粒.txt

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總價(jià)格:¥2000