插入片段

  • 网络insert;Insert Fragment;Insert-Size
插入片段插入片段
  1. 转化效率和AD质粒的插入片段的大小表明酵母文库的质量较理想。

    The efficiency of the transformation and the size of the insert fragment satisfied the quality of the yeast library .

  2. 通过PCR鉴定阳性克隆子中cDNA插入片段的大小和酶切验证后测序。

    Positive clones were identified by PCR in the cDNA insert size and restriction enzyme digestion verified and was sent to sequencing .

  3. 经酶切和测序对插入片段进行分析、鉴定。经限制性内切酶和DNA测序分析两个基因是否已经正确连接到真核表达载体中。

    The sequence of fusion gene was examined by enzyme incision and DNA sequencing .

  4. 用定量PCR从杂交阳性融合噬菌斑中分离候选插入片段

    Isolating candidate inserted fragment from positive fused phage clones using quantitative PCR

  5. 结果文库扩增后得到28个阳性克隆,进行菌落PCR分析,均得到200~1000bp插入片段。

    Results The amplified library contained 28 positive clones .

  6. 随机挑选12个克隆,其中11个克隆PCR扩增出插入片段,插入效率约为91%。

    The insertion was amplified in 11 of the 12 randomly selected clones by PCR .

  7. PCR扩增阳性克隆插入片段。

    The inserts were amplified by PCR .

  8. 并对cDNA插入片段进行序列测定。

    The cDNA inserts in the positive clones were PCR amplified and sequenced .

  9. 结果共筛选出13个阳性克隆,PCR扩增出特异的插入片段。

    Results Thirteen positive clones were obtained after three rounds of immunoscreening , and all amplified by PCR .

  10. PCR结果表明,这些重组腺病毒DNA的插入片段大小是正确的。

    DNA , respectively . The PCR results showed that the insertions of the recombinant adenoviruses were of the right size .

  11. 菌落PCR分析结果表明,95%左右的阳性克隆含有大小200~700bp的插入片段。

    Colony PCR analysis showed that 95 % of the positive clones containing the size of 200 ~ 700 bp of the inserts .

  12. 结果随机挑取50个直径>1mm的白色克隆进行PCR扩增分析,其中47个克隆有插入片段,克隆阳性率为94%。

    Results Random analysis of 50 white clones with PCR amplification showed that 47 clones contained inserted fragments . The positive rate was 94 % .

  13. 文库的滴度、重组率及插入片段的大小是鉴定cDNA文库质量的重要指标。

    Titre , recombination rate and the size of the inserting fragment are important index for the quality of the cDNA library .

  14. 结果PCR产物琼脂糖电泳结果显示:在预期位置有阳性条带;序列分析和酶切结果证实插入片段序列正确。

    Result A positive band was formed when product of PCR electrophresed on agar gel and inserted fragment was confirmed correctly by sequencing and enzyme digestion analysis .

  15. 抗冻肽cDNA插入片段经杂交证实后,对其进行了酶谱分析,核酸序列测定。

    After confirmation of the insert segment of the cDNA of antifreeze protein gene , the zymogram was detected and the sequence of the nucleotides was determined .

  16. 重组子经EcoRⅠ酶切验证显示:重组质粒均含有外源DNA插入片段。

    The results after digested by restriction enzyme EcoR ⅰ revealed that the recombinants which had been picked out contained foreign DNA fragments .

  17. 结果文库容量为1.9×106个重组子,文库中cDNA插入片段大小介于0.4×103~6.5×103bp。

    Results There are 1.9 × 10 6 recombinants in this library . The cDNA fragments ranged between 0.4 × 10 3 bp and 6.5 × 10 3 bp .

  18. 进一步DNA测序结果显示插入片段与tsbp编码序列一致,阅读框架完整,并且无移码。

    Further DNA sequencing manifested that the insertion element was tsbp sequence with complete reading frame and no frame shift .

  19. 其中减数分裂时期正向消减文库共获得276个重组菌落,经菌液PCR鉴定获得了229个阳性插入片段,片段大小均在100~1000bp之间。

    276 recombinant clones were obtained from forward subtractive cDNA library of meiosis period , 229 of which were positive insertional fragments with the average sizes of 100 ~ 1000 bp by PCR identification .

  20. 对重组质粒的分析表明,插入片段的序列与发表的VDR基因编码序列相同。

    The sequence of the insert in the plasmid was identical to the published coding-region sequence of VDR gene .

  21. 结果表明,以λ噬菌体DNA为模板直接测序比PCR产物经回收后为模板进行测序,其目标克隆的平均插入片段长度要长,但反应成功率低。

    The results showed that the insert fragment length of target clones as λ phage DNA template directly sequencing was longer than that of PCR products after recycling , but a lower succeeding ratio for sequencing reaction .

  22. 联合蓝白斑和菌落PCR方法筛选含插入片段的阳性克隆,进行测序和同源性分析,并经Northern杂交技术检测基因的表达。

    Clones with inserts were selected with combination of α - complementary phenomenon and colony PCR method . The sequencing and homology analysis were then performed and the mRNA expression levels were measured by Northern blotting .

  23. 随机选取50个克隆,用位于pRAC质粒多克隆位点两侧的测序引物进行菌落PCR扩增,检测文库插入片段的分布情况。

    50 clones were selected randomly and the colony PCR amplification was used to detect the distribution of library inserts with pRAC sequencing primers .

  24. 方法:以弓形虫RH株速殖子感染大鼠血清作为探针筛选弓形虫cDNA文库,对阳性克隆的插入片段进行PCR扩增及DNA序列测定。

    Methods Rats were infected with Toxoplasma gondii RH strain and their serum was used as a probe to screen Toxoplasma gondii tachyzoite cDNA expression libraries . The positive clones were analyzed by PCR amplification and DNA sequencing .

  25. 插入片段中存在一个RNA聚合酶Ⅲ启动子及AluⅠ内切酶识别位点,所以该片段可能为Alu成分。

    According to the RNA polymerase ⅲ promoter structure and Alu ⅰ restriction enzyme site in the inserted fragment , it should be regarded as an Alu element .

  26. 对该文库特性研究表明,该文库包含了2.15×106个单个克隆,背景低于100pfu/μgDNA,插入片段平均大小约为17kb,证明是一个较为完整的脐橙基因组DNA文库。

    A DNA library with 2 . 15 × 106 individual clones and a low background at 100 pfu / μ g DNA was obtained . The average length of inserts is about 17 kb . The library was proved to be standard and representative .

  27. 结果:构建了2×109大容量天然人源Fab抗体库,经核苷酸序列分析,证实插入片段为Fab基因片断。

    Results : A large naive human Fab phage-display library consisting of 2 × 109 clones was successfully constructed . The sequencing result demonstrated that it was a human Fab gene .

  28. 质粒经NotI酶切鉴定插入片段大小。

    Inserts size were identified by Plasmid NotI digestion .

  29. 在根据插入片段酶切指纹图谱对SSH文库中的414个阳性克隆进行分类的基础上,从12个出现频率较高的类型中各选一个克隆测序。

    Based on the restriction enzyme-digested fingerprinting patterns , 414 positive SSH clones randomly picked from the library were classified into 73 groups , one clone from each of the 12 groups with the higher frequencies was sequenced .

  30. 对经EcoRⅠ酶切鉴定为阳性的重组表达质粒测序,结果显示插入片段大小、方向、碱基匹配与预期一致。

    After sequencing the positive recombinant plasmid which was identified by EcoR ⅰ, results showed that the inserted fragment was right in length , direction and base matching .