基因敲除技术在微生物中的应用

随着分子生物学技术的发展,基因敲除技术越来越广泛地应用于动植物、微生物领域,成为研究生物基因功能最有力的工具之一。基因敲除技术在改造动植物、微生物基因组、研究发育生物学、鉴定新基因新功能、育种以及医疗领域都有应用价值。针对微生物方面,对实现基因敲除的各种原理方法,RecA系统同源重组法, Red系统同源重组法,基于自杀载体的同源重组法,基于温敏型质粒的同源重组法, CRISPR/Cas系统介导的基因敲除方法进行了总结,比较各自的优缺点,并提供一些成功案例以及各种方法相关的发明专利,以期对了解基因敲除技术的方法与发展提供参考。     

一种基于线性DNA片段同源重组的嗜盐古菌高效基因敲除系统

随着功能基因组学研究的深入发展,基因敲除技术日益成为基因功能研究的重要手段。嗜盐古菌Haloferax volcanii易于培养,是研究古菌基因功能的良好模式菌株。虽然现已开发了多种嗜盐古菌的遗传操作系统,但基因敲除成功率不十分理想。这些遗传操作方法基于pyrE筛选标记,利用携带同源片段的环状质粒与基因组同源片段间的两次同源重组,敲除目的基因。由于基于环状质粒和pyrE筛选标记的经典同源重组敲除方法在二次重组时,普遍存在回复到野生型菌株的可能,导致二次重组子中敲除目的基因的阳性菌株比例较低。为了克服传统同源重组技术的上述缺陷,文章建立了基于线性DNA片段的同源重组技术。该方法通过一次重组在目标基因的下游引入一段上游同源片段和pyrE标记,从而限定二次重组的发生部位只能在两段上游同源片段之间,发生二次重组的重组子理论上都敲除了目标基因。利用该方法,文章成功敲除了嗜盐古菌Haloferax volcanii的xpd2基因,阳性克隆率达65%。这种线性DNA片段重组法为嗜盐古菌的基因敲除提供了一种高效策略,便于嗜盐古菌的基因改造。     

工业微生物代谢途径调控的基因敲除策略

基因敲除技术是一项重要的分子生物学技术,在工业微生物代谢工程中具有广泛应用。以下从基因敲除技术的遗传重组原理出发,总结了基因敲除策略的类型、特征和应用,重点介绍了采用线性双链DNA的λRed同源重组系统、使用环状质粒载体介导的单交换或双交换同源重组策略以及采用转座酶介导的转座重组等几种主要的基因敲除方法,进一步展望了基因敲除技术的发展前沿和应用前景。     

2型猪链球菌中国强毒株05ZYH33 sao基因敲除突变株的构建及其生物学功能

构建2型猪链球菌(Streptococcus suis serotype 2,S.suis 2)中国强毒株05ZYH33的sao基因敲除突变株。构建中间为壮观霉素抗性基因,两侧为sao编码基因上下游同源序列的基因敲除载体,同源重组筛选sao基因敲除突变株。PCR、RT-PCR、Western Blot对疑似突变株进行验证,实验结果均证实sao基因完全被spc抗性基因替代,成功构建了突变株05ZYH33-sao。对野生型菌株和突变株进行菌落溶血活性、生长特性、小鼠致病性比较,结果表明sao基因的敲除并未使野生型菌株在以上三方面产生明显的变化。筛选获得的05ZYH33 sao基因突变株为进一步研究sao基因在05ZYH33致病过程中的作用奠定了基础。     

用Red/ET重组酶构建基因打靶载体

基因敲除的小鼠模型是研究基因功能的一种重要资源。采用常规分子克隆的方法建立基因敲除的打靶载体存在构建效率低和难以获得长片段同源臂的缺点。因此快速高效地构建打靶载体,已成为获得特定基因敲除动物模型的关键环节。为研究Resp18未知功能分泌肽基因,应用一种新的DNA工程平台——Red/ET同源重组技术来构建其打靶载体,并比较了这一方法在构建不同长度同源臂中的效率。研究表明,Red/ET重组方法构建打靶载体具有很高的效率,可以获得较长的同源臂,并且不会引入突变,有助于获得更高的打靶效率。因此Red/ET重组为构建打靶载体提供了一种新的可靠的方法。     

Ⅱ型猪链球菌二元信号转导系统2148hk/rr基因敲除突变体的构建

构建猪链球菌2型(Streptococcus suis type 2)强毒株05ZYH33二元信号转导系统2148hk/rr基因敲除突变体.构建中间为壮观霉素抗性基因,两侧为2148hk/rr编码基因上、下游同源序列的基因敲除质粒,通过同源重组筛选2148hk/rr编码基因敲除突变体.PCR分析和Southern杂交结果均显示2148hk/rr编码基因完全被壮观霉素抗性基因替代,基因敲除突变体构建成功.筛选获得05ZYH33二元信号转导系统2148hk/rr基因敲除突变体,为阐明该调控系统在猪链球菌致病过程中的作用奠定了基础.     

利用细菌人工染色体同源重组对小鼠基因进行条件型敲除

目的:探索通过细菌人工染色体(BAC)同源重组系统构建条件基因敲除载体的高效率方法,提高条件基因敲除小鼠(Flox小鼠)的构建效率。方法:利用作者自己构建的噬菌体重组酶系统,通过BAC同源重组进行条件型基因敲除载体构建工作。首先通过亚克隆构建了一系列载体含有同源臂的靶向质粒,线性化后,打靶片段经电穿孔法转入大肠杆菌内,与相应的BAC同源重组,再经过三步同源重组和一步位点特异性重组,构建小鼠条件型基因敲除载体。结果:高效率构建了小鼠基因的最终条件基因敲除载体。结论:通过BAC同源重组高效构建条件基因敲除载体,为条件基因敲除载体的构建提供了全新思路,并为FLox小鼠的建立,及相应基因在发育、生理、致病机制等方面的功能研究奠定了基础。     

丙酸杆菌基因敲除体系的构建及其应用

目的 丙酸杆菌基因敲除体系的构建及其验证.方法 利用PCR技术扩增丙酸杆菌hemE基因上、下游约500 bp左右片段,构建由上下游同源臂及hygB抗性基因组成的打靶质粒pPK705-arms-hygB.将打靶质粒转入丙酸杆菌感受态细胞,利用同源重组技术定向敲除hemE基因,并通过连续传代培养,消除外源质粒.最后,利用PCR技术验证丙酸杆菌染色体和打靶质粒发生同源重组.结果 成功敲除了丙酸杆菌hemE基因.结论 打靶质粒pPK705-arms-hygB能够与宿主基因组DNA发生重组,对稳定地改善其整个代谢途径的研究奠定了方法学基础.     

Ⅱ型猪链球菌二元信号转导系统2148hk/rr基因敲除突变体的构建

构建猪链球菌2型(Streptococcus suis type 2)强毒株05ZYH33二元信号转导系统2148hk/rr基因敲除突变体。构建中间为壮观霉素抗性基因, 两侧为2148hk/rr编码基因上、下游同源序列的基因敲除质粒, 通过同源重组筛选2148hk/rr编码基因敲除突变体。PCR分析和Southern杂交结果均显示2148hk/rr编码基因完全被壮观霉素抗性基因替代, 基因敲除突变体构建成功。筛选获得05ZYH33二元信号转导系统2148hk/rr基因敲除突变体, 为阐明该调控系统在猪链球菌致病过程中的作用奠定了基础。     

Ku基因在微生物中的研究进展

ku基因介导的非同源末端连接(NHEJ)途径是DNA双链断裂(DSBs)的一种修复机制,它不依赖于同源重组,且通过与之竞争而削弱同源重组。由于ku基因在生物进化过程中的高度保守性,其功能在很多微生物中已经得到研究,尤其在丝状真菌中,将ku基因敲除,在NHEJ途径缺陷的背景下,同源重组发挥主要作用,基因敲除的频率大为提高,从而方便了对基因功能的研究。     

BCL2-CISD2

CISD2, an ER BCL2-associated autophagy regulator also known as NAF-1, is responsible for the human degenerative disorder Wolfram Syndrome 2. In order to interrogate the physiological role of CISD2 we generated and characterized the Cisd2 gene deletion in mice. Cisd2 null mice manifest significant degeneration in skeletal muscle tissues, which is accompanied with augmented autophagy, dysregulated Ca²⁺ homeostasis and elongated mitochondria. Our findings describe a novel role for BCL2-CISD2 in the homeostatic maintenance of skeletal muscle. It remains to be elucidated how and if the antagonism of the BECN1 autophagy-initiating complex and modulation of ER Ca²⁺ homeostasis by BCL2-CISD2 are interconnected.     

Synthesis of [11-2H2], [8-2H2], [7-2H2], [6-2H2], [5-2H2], [4-2H2] and [3-2H2] cis-9-octadecenoates

Deuterated oleates have been synthesized by semihydrogenation of acetylenic intermediates. [11-²H₂]Oleate was prepared by two-carbon chain extension of the C₁₆ alcohol obtained from [1-²H₂]octyl bromide and 7-octyn-1-ol. [8-²H₂] and [7-²H₂]oleates were both prepared from dimethyl suberate, tetradeutero intermediate C₁₆ alcohols were synthesized from [1,8-²H₄] and [2,7-²H₄]octane diols by monobromination, conversion to deuterated 9-decyn-1-ols and reaction with octyl bromide. Oxidation gave [8-²H₂]-9-octadecynoate and [2,7-²H₂]-9-octadecynoate, after semihydrogenation of the latter, deuterons at C-2 were removed by exchange with aqueous alkali. [6-²H₂] and [5-²H₂]oleates were obtained from methyl 5-tetradecynoate, semihydrogenation, deuterium exchange at C-2 and two malonate extensions gave [6-²H₂]oleate; reduction with lithium aluminum deuteride, two malonate extensions and semihydrogenation gave the [5-²H₂] ester. [4-²H₂] and [3-²H₂]oleates were both obtained from methyl 7-cis-hexadecenoate, exchange of the α protons and chain extension gave the [4-²H₂] ester and reduction with lithium aluminum deuteride and chain extension gave the [3-²H₂] ester.     

Synthesis and physicochemical properties of 2'-deoxy-2',2'-difluoro-beta-D-ribofuranosyl and 2'-deoxy-2',2'-difluoro-alpha-D-ribofuranosyl oligonucleotides

We present procedures for nucleoside and oligonucleotide synthesis, binding affinity (Tm) and structural analysis (CD spectra) of 2'-deoxy-2',2'-difluoro-alpha-D-ribofuranosyl and 2'-deoxy-2',2'-difluoro-beta-D-ribofuranosyl oligothymidylates. Possible reasons for the thermal instability of duplexes formed between these compounds and RNA or DNA targets are discussed.     

Stereospecific 2'-amination and 2'-chlorination of adenosine by Actinomadura in the biosynthesis of 2'-amino-2'-deoxyadenosine and 2'-chloro-2'-deoxycoformycin

2'-Amino-2'-deoxyadenosine and 2'-chloro-2'-deoxycoformycin (2'-CldCF) are two nucleoside antibiotics produced by Actinomadura. The biosynthesis of these two nucleoside antibiotics has been studied by the addition of [U-14C]adenosine with or without unlabeled adenine to cultures of Actinomadura. By this experimental approach, it is possible to demonstrate that adenosine is the direct precursor for the biosynthesis of 2'-amino-2'-deoxyadenosine and 2'-CldCF. These conclusions are based on the observation that the percentage distribution of 14C in the aglyconic and pentofuranosyl moieties of 2'-amino-2'-deoxyadenosine and 2'-CldCF were similar to the distribution of 14C in the adenine and ribosyl moieties of the [U-14C]adenosine (i.e., 48:52) added to cultures of Actinomadura. Experimentally, the percentage distribution of 14C in the (i) adenine:2-amino-2-deoxy-beta-D-ribofuranose of 2'-amino-2'-deoxyadenosine is 51:49; (ii) 8-(R)-3,6,7,8-tetrahydroimidazo[4,5-d]-[1,3-diazepin-8-o1]:2 -chloro-2- beta-D-ribofuranose of 2'-CldCF is 45:55; and (iii) adenine:ribose of the adenosine isolated from the RNA of Actinomadura is 42:58. Further proof that adenosine is the direct precursor for the biosynthesis 2'-amino-2'-deoxyadenosine and 2'-CldCF was demonstrated by the addition of 75 mumol of unlabeled adenine together with [U-14C]adenosine to nucleoside-producing cultures of Actinomadura. The percentage distribution of 14C in the aglycon and the sugar moieties of 2'-amino-2'-deoxyadenosine and 2'-CldCF were 46:54 and 47:53, respectively; the percentage distribution of 14C in the adenine and ribose moieties of the adenosine isolated from the RNA of Actinomadura was 51:49. These data show that the hydroxyl on C-2' of the ribosyl moiety of adenosine undergoes a replacement by a 2'-amino or a 2'-chloro group to form 2'-amino-2'-deoxyadenosine or 2'-CldCF with retention of stereconfiguration at C-2'. Finally, Actinomadura can utilize inorganic chloride from the medium as demonstrated by the isolation of [36Cl]2'-CldCF following the addition of [36Cl]chloride to the culture medium. Mechanisms for the regioselective modification of the C-2' hydroxyl group and stereospecific insertion of the amino and chloro groups are discussed.     

Stereospecific formation of alpha-hydroxycarboxylato oxo peroxo complexes of vanadium(V). Crystal structure of (NBu4)2[V2O2(O2)2(L-lact)2] x 2H2O and (NBu4)2[V2O2(O2)2(D-lact)(L-lact)] x 2H2O

An overview of structurally characterized alpha-hydroxycarboxylatodioxo- and alpha-hydroxycarboxylatooxoperoxovanadates(V) is presented and the geometric parameters of the V2O2 bridging core are discussed. The first case of a stereospecific formation of oxoperoxovanadates(V) is reported: The crystal structures of the isomeric compounds (NBu4)2[V2O2(O2)2(L-lact)2] x 2H2O and (NBu4)2[V2O2(O2)2(D-lact)(L-lact)] x 2H2O (lact = C3H4O3(2-), the anion of the lactic acid) differ mainly in the arrangement of the V2O2 core and in mutual orientation of the V=O bonds. The complexes with achiral ligands adopt the same structural type as the complexes formed from a racemic mixture of a chiral ligand, while the structure obtained using an enantiopure L,L-hydroxycarboxylate is different.     

Stereoselective Synthesis of 2-Amino-2-deoxy-d-arabinose and 2-Deoxy-d-ribose

An efficient method for the stereoselective synthesis of 2-amino-2-deoxy-d-arabinose and 2-deoxy-d-ribose is described.

The key step in this method was accomplished by the nucleophilic addition of methyl isocyanoacetate to 2,3-O-isopropylidene-d-glyceraldehyde with high erythro-selectivity (nearly 100%).

Subsequent intermolecular cyclization predominantly gave the desired oxazoline derivative (trans-form), in which two new chiral centers were formed. The oxazoline derivative was efficiently converted to both 2-amino-2-deoxy-d-arabinose and 2-deoxy-d-ribose.