人尿激酶原cDNA片段克隆及鉴定

尿激酶(UK)是一种在人肾合成并由人尿释放的一种纤溶酶原激活剂,可用于治疗血拴病。现已发现有四种不同分子形式的尿激酶。有关尿激酶原cDNA的克隆及表达已有文献报道。本文报道经反转录途径获得一个含人尿激酶原cDNA片段的克隆,并进行了酶切及核苷酸序列分析鉴定。

构建转CgA基因反向cDNA片段小鼠模型

为了制作ＣｇＡ基因反义ＲＮＡ转基因小鼠，构建了质粒ｐＣＡＳ２Ｃ，并把ｐＣＡＳ２Ｃ中完整 的反义表达框显微注射入小鼠受精卵的雌原核中，随后将注射过ＤＮＡ的受精卵移植入假 孕鼠的输卵管中。假母所产子一代都用ｐ１和ｐ４引物对鼠尾基因组ＤＮＡ进行ＰＣＲ检测，选 出２只首建鼠（ＰＣＲ阳性）。首建鼠与正常鼠杂交后得到Ｆ１代小鼠，经ＰＣＲ方法筛选出来的 阳性Ｆ１代鼠雌雄自交产生Ｆ２代。为了检测Ｆ２代鼠的基因型，将ＰＣＲ方法鉴定为阳性的 Ｆ２代 小鼠分别与正常小鼠回交。只有回交后所得后代ＰＣＲ检测结果全为阳性的Ｆ２代个体才是 转基因纯合鼠。这样分别得到两只转基因首建鼠的纯合个体。转基因小鼠脑总ＲＮＡ经 ＲＴ－ＰＣＲ反应后可产生３００ｂｐ的产物，证明转基因小鼠中转入的反义基因已经转录。以上结 果说明转入的ｐＣＡＳ２Ｃ反义表达框已经整合到转基因小鼠的基因组中并遗传给后代，而且 已经转录。

Isolation of 24 novel cDNA fragments from microdissected human chromosome band

The strategy of isolating the band-specific expression fragments from a probe pool generated by humanchromosome microdissection was reported. A cliromosome 14q24.3 band-specific single copy DNA pool was constructed based on this probe pool. Using total DNA of the pool as probe to hybridize the human marrow cDNA library, 68 primary positive clones were selected from 5 ×105 cDNA clones. Among these primary clones, 32 secondary clones were obtained after second-round screening and designed as cFD14-1～32. Finally, 24 band-specific expression fragments were identified from these 32 positive clones by DNA hybridization. Those band-specific clones can hybridize to both 14q24.3 DNA and human genomic DNA but cann’t hybridize to 17q11～12 DNA. Partial sequences of 13 fragments of them were sequenced and identified as novel cDNA sequences , and these sequences were proved to have some homology with known genes in NCBI database. Analysis of expression spectrum of cFD14-1 suggested that the cDNA fragments thus obtained should be used to isolate the genes can not been cloned in 14q24.3region.