MIP gene

  • 文章类型: Journal Article
    先天性白内障是导致儿童不可逆视力障碍的主要原因,遗传因素在其发展中起着重要作用。在这项研究中,靶向外显子组测序揭示了一个新的单碱基缺失突变的MIP(c.301delG;p.Ala101Profs*16),在一个中国家庭中与先天性点状白内障分离.疏水性,通过生物信息学分析,预测截短MIP的二级和三级结构会影响蛋白质的功能。当将MIP-WT和MIP-Ala101fs表达构建体单独转染到HeLa细胞中时,发现mRNA水平没有显着差异,与野生型MIP相比,突变体的蛋白质水平显着降低。免疫荧光图像显示MIP-WT主要位于质膜,而MIP-Ala101fs蛋白被异常捕获在细胞质中。此外,与MIP-WT相比,MIP-Ala101fs的细胞间粘附能力和细胞间通讯特性均显着降低(均*p<0.05)。这是与常染色体显性遗传先天性白内障相关的MIP基因c.301delG突变的首次报道。我们认为白内障是由突变MIP导致的蛋白质表达减少和细胞间粘附减少引起的。突变蛋白的运输受损或不稳定,以及受损的细胞间通讯可能是突变的并发结果。结果扩展了MIP的遗传和表型谱,并有助于更好地了解先天性白内障的分子基础。
    Congenital cataracts are the leading cause of irreversible visual disability in children, and genetic factors play an important role in their development. In this study, targeted exome sequencing revealed a novel single-base deletional mutation of MIP (c.301delG; p.Ala101Profs*16) segregated with congenital punctate cataract in a Chinese family. The hydrophobic properties, and secondary and tertiary structures for truncated MIP were predicted to affect the function of protein by bioinformatics analysis. When MIP-WT and MIP-Ala101fs expression constructs were singly transfected into HeLa cells, it was found that the mRNA level showed no significant difference, while the protein level of the mutant was remarkably reduced compared to that of the wild-type MIP. Immunofluorescence images showed that the MIP-WT was principally localized to the plasma membrane, whereas the MIP-Ala101fs protein was aberrantly trapped in the cytoplasm. Furthermore, the cell-to-cell adhesion capability and the cell-to-cell communication property were both significantly reduced for MIP-Ala101fs compared to the MIP-WT (all *p < 0.05). This is the first report of the c.301delG mutation in the MIP gene associated with autosomal dominant congenital cataracts. We propose that the cataract is caused by the decreased protein expression and reduced cell-to-cell adhesion by the mutant MIP. The impaired trafficking or instability of the mutant protein, as well as compromised intercellular communication is probably a concurrent result of the mutation. The results expand the genetic and phenotypic spectra of MIP and help to better understand the molecular basis of congenital cataracts.
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  • 文章类型: Journal Article
    Root and collar rot disease caused by Phytophthora capsici (Leonian) is one of the most serious diseases in pepper, Capsicum annuum L. Knowledge about resistant genes is limited in pepper accessions to P. capsici. In this study, a diverse collection of 37 commercial edible and ornamental genotypes, and implication of seven novel candidate DEGs genes (XLOC_ 021757, XLOC_021821, XLOC_012788, XLOC_011295, XLOC_021928, XLOC_015473 and XLOC_000341) were up-regulated on resistant and susceptible pepper cultivars, through real-time polymerase chain reaction (qPCR) at transplanting and maturing stages. All seven related defense-gene candidates were up-regulated in all inoculated accessions to P. capsici, but these genes were highly expressed in resistant ones, 19OrnP-PBI, 37ChillP-Paleo, and 23CherryP-Orsh. The transcriptional levels of the seven related candidate DEGs were 5.90, 5.64, 5.62, 5.18, 3.94, 3.69, 3.16 folds higher in the resistant pepper genotypes, than the control ones, non-inoculated genotypes respectively. The candidate genes expressed herein, will provide a basis for further gene cloning and functional verification studies, and also will aid in an understanding of the regulatory mechanism of pepper resistance to P. capsici.
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  • 文章类型: Journal Article
    军团菌种类广泛存在于天然水源和人造水环境中,以及淡水。本研究是由于缺乏有关伊朗西南部阿瓦士市水源中军团菌属流行的研究而进行的。在这项研究中,巨噬细胞感染性增效剂(mip)基因测序用于鉴定从不同水源分离的各种军团菌。在这项研究中,收集144个水样并接种在缓冲木炭-酵母提取物(BCYE)琼脂和改良的Wadowsky-Yee(MWY)培养基上。从阳性培养物中提取DNA。通过扩增16SrRNA基因的654bp片段来确认军团菌物种。通过PCR扩增所有分离物的mip基因并纯化用于测序。通过jPHYDIT软件版本1分析mip基因序列。结果显示军团菌的患病率为13.9%(20/144)。在阿瓦士市的水源,伊朗西南部。对mip基因序列的分析显示,在20个军团菌分离株中,13株(54.1%)肺炎杆菌阳性,5个分离株(20.8%)对苦力乳杆菌呈阳性,DumoffiL.和FairfieldensisL.(4.1%)。根据我们的研究,水源中军团菌的发生可能对卫生系统构成危害,尤其是在医院中。因此,健康计划人员对这些水源进行定期监测可能有助于降低军团菌的风险。感染。
    Legionella species are widespread in natural water sources and man-made aqueous environments, as well as fresh-water. The present study was conducted owing to the lack of research regarding the prevalence of Legionella spp in the water sources of Ahvaz city in southwest Iran. In this study the macrophage infectivity potentiator (mip) gene sequencing was used for identification of various Legionella species isolated from different water sources. In this study, 144 water samples were collected and inoculated on the buffered charcoal-yeast extract (BCYE) agar and modified Wadowsky-Yee (MWY) medium. The DNA was extracted from positive cultures. The Legionella species were confirmed by amplifying a 654 bp fragment of the 16S rRNA gene. The mip gene of all isolates were amplified by PCR and purified for sequencing. The mip gene sequences were analyzed by jPHYDIT software version 1. The results showed a 13.9% (20/144) prevalence of Legionella spp. in water sources of Ahvaz city, southwest Iran. Analyzing of the mip gene sequences showed, out of 20 Legionella isolates, 13 isolates (54.1%) were positive for L. pneumophila, 5 isolates (20.8%) were positive for L. worsleinsis, one isolates for each one of L. dumoffi and L. fairfieldensis, (4.1%). According to our research, the occurrence of Legionella spp in water sources could be a hazard for the health systems especially in the hospitals. The regular monitoring of these water sources by health planners may therefore be useful for decreasing the risk for Legionella spp. infections.
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  • 文章类型: Journal Article
    军团病是一个重要的公共卫生问题,可以导致大量的死亡率和发病率。军团菌检测方法的不确定性可能会损害军团菌疾病风险估计。这项研究的目的是通过培养检测有呼吸道症状的住院患者的呼吸道标本中的肺炎杆菌。PCR,和环介导等温扩增(LAMP)方法。
    痰液和支气管肺泡灌洗样本取自阿瓦士教学医院的肺炎患者,伊朗从2016年6月到2017年3月。军团菌的分离.通过直接在缓冲木炭-酵母提取物和改良的Wadowsky-Yee琼脂培养基上培养样品来完成。然后,进行PCR和LAMP测定,以通过其mip基因在呼吸道标本中检测嗜肺乳杆菌。
    共收集100个呼吸道标本。我们的结果表明,1%的样品对军团菌属呈培养阳性。,3%和7%的样本在PCR和LAMP分析中使用mip基因检测肺炎杆菌阳性,分别。
    在肺部感染性疾病的诊断中应考虑军团病。此外,LAMP测定法是一种比常规方法更快速,具有更高的灵敏度和特异性的方法,如PCR和培养,用于军团病的实验室诊断。
    UNASSIGNED: Legionnaires\' disease is an important public health problem that can cause substantial mortality and morbidity. Legionnaires\' disease-risk estimation may be compromised by uncertainties in Legionella-detection methods. The aim of this study was the detection of L. pneumophila in respiratory specimens of hospitalized patients with respiratory symptoms by culture, PCR, and loop-mediated isothermal amplification (LAMP) methods.
    UNASSIGNED: Sputum and bronchoalveolar lavage samples were obtained from patients with pneumonia admitted to teaching hospitals in Ahvaz, Iran from June 2016 to March 2017. Isolation of Legionella spp. was done by culturing the samples directly onto buffered charcoal-yeast extract and modified Wadowsky-Yee agar medium. Then, PCR and LAMP assays were performed for detection of L. pneumophila via its mip gene in respiratory specimens.
    UNASSIGNED: A total of 100 respiratory specimens were collected. Our results showed that 1% of the samples were culture positive for Legionella spp., and 3% and 7% of samples were positive for L. pneumophila using the mip gene on PCR and LAMP assays, respectively.
    UNASSIGNED: Legionnaires\' disease should be considered in the diagnosis of pulmonary infectious diseases. Also, the LAMP assay is a faster method with higher sensitivity and specificity than conventional methods, such as PCR and culture, for laboratory diagnosis of Legionnaires\' disease.
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  • 文章类型: Journal Article
    Legionella pneumophila is the primary respiratory pathogen and mostly transmitted to human through water cooling systems and cause mild to severe pneumonia with high mortality rate especially in elderly both in hospitals and community. However, current Legionella risk assessments may be compromised by uncertainties in Legionella detection methods. Here, we investigated the presence of L. pneumophila mip gene in water samples collected from different hospitals cooling towers, nursing homes and building/hotels water coolants from two geographical locations of Iran (Kerman and Bam cities) during summer season of 2015 by both nested and real-time PCR methods. Analysis of the 128 water samples for presence of the mip gene by nested-PCR revealed, 18 (23%) positive cases in Kerman and 7(14%) in Bam. However, when samples were tested by real-time PCR, we identified 4 more new cases of L. pneumophila in the hospitals as well as nursing homes water systems that were missed by nested-PCR. The highest rate of contamination was detected in water obtained from hospitals cooling towers in both the cities (p≤0.05). Dendrogram analysis and clonal relationship by PCR-base sequence typing (SBT) of the L. pneumophila genomic DNAs in Kerman water samples showed close clonal similarities among the isolates, in contrast, isolates identified from Bam city demonstrated two fingerprint patterns. The clones from hospital water samples were more related to the L. pneumophila serogroup- 1.
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