猪肺炎支原体基因组DNA文库的构建

将猪肺炎支原体Z菌株接种于A2 6液体培养基中培养 ,在收获菌体细胞后 ,提取和纯化其基因组DNA。并经EcoRI大量酶切获得 4 .0～ 8.0kb的DNA片段 ,与λgt11载体臂连接为重组λDNA ,然后进行包装 ,感染于Y10 90宿主菌 ,构建了猪肺炎支原体基因组DNA文库 ,并得以表达。

人核蛋白P68 cDNA基因克隆及全序列测定

靠人工合成4个混合寡聚核苷酸探针,从一个人胎盘λgt11 cDNA库中筛选到含有p68 cDNA基因的阳性噬菌斑。经次克隆得到含p68 cDNA基因的pBRB_(T7)—p68质粒。用末端终止法对此cDNA基因进行了全序列测定。分析结果证明得到的p68 cDNA基因含有2287个核苷酸,具有一个可阅读框架,共编码614个氨基酸。其5′端非编码区含有130个碱基。3′端非编码区含有315个碱基,比已发表的3′端非编码区多23个碱基。

用λgt11载体构建人脑胶质瘤基因文库

自人脑胶质瘤手术标本中提取mRNA,逆转录合成cDNA,在T_4DNA 连接酶作用下,与一头是平末端,另一头是EcoR I 粘性末端、内含Not I 切点的插头相连,经T_4多聚核苷酸激酶磷酸化后,再与脱磷酸处理过的λgt11 臂连接,形成重组λgt11DNA。体外包装,构建了一个库容量含1.02×10~6重组子的人脑胶质瘤cDNA 基因文库。克隆效率为1.08×10~7pfu/μg cDNA。重组百分比为96.2%。

水稻小穗cDNA文库的构建

用蛋白酶K-苯酚法,从开花后7～14天的水稻小穗,抽提纯化出有生物学活性的总poly(A)^+RNA,在AMV逆转录酶作用下,将它反转录合成第一链cDNA,并在DNA聚合酶I和核酸酶SI作用下,合成双链cDNA。cDNA经甲基化修饰,通过EcoRI接头与表达型载体λgtll DNA连接,经离体包装构建出水稻开花后小穗cDNA文库。该文库的复杂度为2.4 ×10~6pfu,重组体的比率为14％。

普氏立克次体基因文库的构建

普氏立克次体Breinl株(Rickettsia prowazekii strain Breinl)经6种平端内切酶部分消化,行EcoRI位点甲基化,加上EcoRI接头,与去磷酸化的λgtll DNA-EcoRI臂连接,体外包装后感染E.coil Y1090,建成含2.18X 10~4重组子的表达型普氏立克次体基因文库,随机选择的白斑噬菌体DNA经酶切鉴定表明均含大小不等的插λDNA片段。

人胎肝cDNA文库的构建

从水囊引产的4～5个月孕龄胎儿肝脏中提取mRNA,合成单、双链CDNA,用离心式柱层析去除短的cDNA片段,加上EcoRI接头,与去磷酸化的λgt 11 DNA-EcoRI长、短臂连接,体外包装后感染Y1090,建成含4.05×10~5重组子的表达型人胎肝cDNA文库。白斑噬菌体DNA经酶切鉴定表明均含1kb以上大小不等的CDNA片段。

Construction and primary characterization of Echinococcus multilocularis protoscolex cDNA expression library

Objective To construct a λgt11 cDNA expression library of Echinococcus multilocularis protoscolex isolated in China. Methods Echinococcus multilocularis protoscolex mRNA was extracted using a Quickprep MicromRNA purification kit based on combining of the disruptive and protective properties of guanidinium thiocyanate (GTC) with the speed and selectivity of oligo (dT)-cellulose chromatography in a spum-column with some modification. Purified mRNA (1.8 μg) was submitted to reverse transcription using random hexamers ［pd(N6)］. The double-strand blunt-ended cDNAs were ligated with an EcoRI/NotI adaptor to form a cohesive EcoRI end. Subsequently the synthesized cDNA was inserted into vector λgt11 EcoRI arms. After being packaged in vitro, λgt11 was put to an infectious bacteria Echinococcus coli (E.coli) strain Y1090; the recombinants were screened by color selection. PCR amplification was performed to evaluate the size of insertion DNA fragments.Results The recombinant ratio was nearly 100% and approximately 1×106 clones could be derived from this λgt11 cDNA library. PCR results indicated that the insertion DNAs were about 1.48 kb. Conclusions A λgt11 cDNA expression library consisting of a million recombinant clones has been constructed from Echinococcus multicularis protoscolex mRNA. Further studies on this library are deserved.

未知cDNA扩增与亚克隆的方法学研究

新型蛋白质的分子克隆基本依靠ｃＤＮＡ文库的筛选，而文库构建的载体多为λｇｔｌｌ。由于λｇｔｌｌＤＮＡ分子量较大（４９ｋｂ），提取过程中多用ＰＥＧ，因此λｇｔｌｌｃＤＮＡ克隆及其直接序列测定极为困难。为克服此困难，作者自行设计了不含克隆位点的一对公用λｇｔｌｌＰＣＲ引物。试用表明，此引物通过改变ＰＣＲ反应条件，可特异性地扩增多种彼此独立的ｃＤＮＡ。经亚克隆后的序列测定表明，用此方法扩增克隆的多种ｃＤＮＡ保留了原有阅读框架和ｐｏｌｙＡ特有序列，因而基本解决了新型蛋白质分子克隆中ｃＤＮＡ亚克隆与序列测定的困难．