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PLoS One. 2014 Jun 4;9(6):e97100. doi: 10.1371/journal.pone.0097100. eCollection 2014.
2
Cytadherence of Mycoplasma pneumoniae induces inflammatory responses through autophagy and toll-like receptor 4.肺炎支原体的细胞黏附通过自噬和 Toll 样受体 4 诱导炎症反应。
Infect Immun. 2014 Jul;82(7):3076-86. doi: 10.1128/IAI.01961-14. Epub 2014 May 5.
3
Experimental infections with Mycoplasma agalactiae identify key factors involved in host-colonization.无乳支原体的实验性感染确定了宿主定殖所涉及的关键因素。
PLoS One. 2014 Apr 3;9(4):e93970. doi: 10.1371/journal.pone.0093970. eCollection 2014.
4
Transposon mutagenesis in Mycoplasma hyopneumoniae using a novel mariner-based system for generating random mutations.利用新型基于 mariner 的系统在猪肺炎支原体中进行转座子诱变以产生随机突变。
Vet Res. 2013 Dec 21;44(1):124. doi: 10.1186/1297-9716-44-124.
5
Ureaplasma parvum serovar 3 multiple banded antigen size variation after chronic intra-amniotic infection/colonization.解脲脲原体 3 血清型慢性羊膜内感染/定植后的多带抗原大小变异。
PLoS One. 2013 Apr 26;8(4):e62746. doi: 10.1371/journal.pone.0062746. Print 2013.
6
RNA helicases: diverse roles in prokaryotic response to abiotic stress.RNA 解旋酶:在原核生物应对非生物胁迫中的多种作用。
RNA Biol. 2013 Jan;10(1):96-110. doi: 10.4161/rna.22638. Epub 2012 Oct 23.
7
Antibiotic susceptibilities and resistance genes of Ureaplasma parvum isolated in South Africa.南非分离的解脲脲原体的抗生素敏感性和耐药基因。
J Antimicrob Chemother. 2012 Dec;67(12):2821-4. doi: 10.1093/jac/dks314. Epub 2012 Aug 9.
8
Comparative genome analysis of 19 Ureaplasma urealyticum and Ureaplasma parvum strains.19 株解脲脲原体和人型支原体的比较基因组分析。
BMC Microbiol. 2012 May 30;12:88. doi: 10.1186/1471-2180-12-88.
9
Evidence for the predominance of a single tet(M) gene sequence type in tetracycline-resistant Ureaplasma parvum and Mycoplasma hominis isolates from Tunisian patients.证据表明,来自突尼斯患者的四环素耐药解脲脲原体和人型支原体分离株中,主要存在单一 tet(M)基因序列型。
J Med Microbiol. 2012 Sep;61(Pt 9):1254-1261. doi: 10.1099/jmm.0.044016-0. Epub 2012 May 11.
10
Serum killing of Ureaplasma parvum shows serovar-determined susceptibility for normal individuals and common variable immuno-deficiency patients.血清杀伤解脲脲原体表明血清型决定了正常个体和常见可变免疫缺陷患者的易感性。
Immunobiology. 2012 Feb;217(2):187-94. doi: 10.1016/j.imbio.2011.07.009. Epub 2011 Jul 12.

使用微型转座子质粒通过微小脲原体转座子诱变进行随机插入和基因破坏。

Random insertion and gene disruption via transposon mutagenesis of Ureaplasma parvum using a mini-transposon plasmid.

作者信息

Aboklaish Ali F, Dordet-Frisoni Emilie, Citti Christine, Toleman Mark A, Glass John I, Spiller O Brad

机构信息

Cardiff University, School of Medicine, Department of Child Health, 5th floor University Hospital of Wales, Cardiff CF14 4XN, UK; Sebha University, Faculty of Engineering and Technology, Medical Laboratory Sciences Department, PO Box 68, Libya.

INRA, UMR 1225, IHAP, 31076 Toulouse, France; Université de Toulouse, INP, ENVT, UMR1225, IHAP, 31076 Toulouse, France.

出版信息

Int J Med Microbiol. 2014 Nov;304(8):1218-25. doi: 10.1016/j.ijmm.2014.09.003. Epub 2014 Sep 26.

DOI:10.1016/j.ijmm.2014.09.003
PMID:25444567
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4450083/
Abstract

While transposon mutagenesis has been successfully used for Mycoplasma spp. to disrupt and determine non-essential genes, previous attempts with Ureaplasma spp. have been unsuccessful. Using a polyethylene glycol-transformation enhancing protocol, we were able to transform three separate serovars of Ureaplasma parvum with a Tn4001-based mini-transposon plasmid containing a gentamicin resistance selection marker. Despite the large degree of homology between Ureaplasma parvum and Ureaplasma urealyticum, all attempts to transform the latter in parallel failed, with the exception of a single clinical U. urealyticum isolate. PCR probing and sequencing were used to confirm transposon insertion into the bacterial genome and identify disrupted genes. Transformation of prototype serovar 3 consistently resulted in transfer only of sequence between the mini-transposon inverted repeats, but some strains showed additional sequence transfer. Transposon insertion occurred randomly in the genome resulting in unique disruption of genes UU047, UU390, UU440, UU450, UU520, UU526, UU582 for single clones from a panel of screened clones. An intergenic insertion between genes UU187 and UU188 was also characterised. Two phenotypic alterations were observed in the mutated strains: Disruption of a DEAD-box RNA helicase (UU582) altered growth kinetics, while the U. urealyticum strain lost resistance to serum attack coincident with disruption of gene UUR10_137 and loss of expression of a 41 kDa protein. Transposon mutagenesis was used successfully to insert single copies of a mini-transposon into the genome and disrupt genes leading to phenotypic changes in Ureaplasma parvum strains. This method can now be used to deliver exogenous genes for expression and determine essential genes for Ureaplasma parvum replication in culture and experimental models.

摘要

虽然转座子诱变已成功用于支原体属,以破坏和确定非必需基因,但之前对脲原体属的尝试均未成功。使用聚乙二醇转化增强方案,我们能够用含有庆大霉素抗性选择标记的基于Tn4001的微型转座子质粒转化微小脲原体的三个不同血清型。尽管微小脲原体和溶脲脲原体之间有很大程度的同源性,但除了一株临床溶脲脲原体分离株外,所有平行转化后者的尝试均失败。采用PCR探测和测序来确认转座子插入细菌基因组并鉴定被破坏的基因。原型血清型3的转化始终仅导致微型转座子反向重复序列之间的序列转移,但一些菌株显示出额外的序列转移。转座子插入在基因组中随机发生,导致从一组筛选克隆中挑选的单个克隆的基因UU047、UU390、UU440、UU450、UU520、UU526、UU582发生独特破坏。还对基因UU187和UU188之间的基因间插入进行了表征。在突变菌株中观察到两种表型改变:DEAD盒RNA解旋酶(UU582)的破坏改变了生长动力学,而溶脲脲原体菌株失去了对血清攻击的抗性,这与基因UUR10_137的破坏和一种41 kDa蛋白表达的丧失一致。转座子诱变成功用于将微型转座子的单拷贝插入基因组并破坏基因,导致微小脲原体菌株出现表型变化。该方法现在可用于递送外源基因进行表达,并确定微小脲原体在培养和实验模型中复制所必需的基因。