Moraxellaceae Infections

Moraxellaceae 感染
  • 文章类型: Journal Article
    镰刀菌枯萎病(FHB)是一种影响某些镰刀菌物种引起的小麦穗的疾病,并导致严重的产量下降和种子污染。从小麦种质中鉴定抗性基因/QTL可能有助于提高小麦生产中的FHB抗性。
    我们的研究评估了205个优良冬小麦品种的FHB抗性。高密度90KSNP阵列用于对组进行基因分型。使用混合线性模型(MLM)对来自三个不同环境的品种进行了全基因组关联研究(GWAS)。
    在15条染色体上发现了66个显着的标记-性状关联(MTA)(P<0.001),解释了5.4%至11.2%的表型变异。在2A染色体上发现了一些涉及FHB抗性的基因组区域中的重要新MTA,3B,5B,6A,7B在来自两个不同环境的品种中,在7B号染色体上发现了6个92cM的MTA。此外,有11个MTA与患病的小穗率和患病的轴率一致相关,因为多效性效应基因座和5D染色体上的D_contig74317_533对FHB抗性是新的。本研究在小麦中预测了八个新的FHB抗性候选基因。三个候选基因,染色体5DS上的TraesCS5D02G006700、TraesCS6A02G013600和TraesCS7B02G370700,6AS,7BL,分别,在通过调节分子内转移酶活性防御FHB方面可能很重要,GTP结合,或小麦中的几丁质酶活性,但需要进一步验证。此外,总共发现了与小麦FHB抗性相关的五个有利等位基因。这些结果为通过标记辅助选择增强小麦育种中的FHB抗性提供了重要的基因/基因座。
    Fusarium head blight (FHB) is a disease affecting wheat spikes caused by some Fusarium species and leads to cases of severe yield reduction and seed contamination. Identifying resistance genes/QTLs from wheat germplasm may help to improve FHB resistance in wheat production.
    Our study evaluated 205 elite winter wheat cultivars for FHB resistance. A high-density 90K SNP array was used for genotyping the panel. A genome-wide association study (GWAS) from cultivars from three different environments was performed using a mixed linear model (MLM).
    Sixty-six significant marker-trait associations (MTAs) were identified (P < 0.001) on fifteen chromosomes that explained the phenotypic variation ranging from 5.4 to 11.2%. Some important new MTAs in genomic regions involving FHB resistance were found on chromosomes 2A, 3B, 5B, 6A, and 7B. Six MTAs at 92 cM on chromosome 7B were found in cultivars from two different environments. Moreover, there were 11 MTAs consistently associated with diseased spikelet rate and diseased rachis rate as pleiotropic effect loci and D_contig74317_533 on chromosome 5D was novel for FHB resistance. Eight new candidate genes of FHB resistance were predicated in wheat in this study. Three candidate genes, TraesCS5D02G006700, TraesCS6A02G013600, and TraesCS7B02G370700 on chromosome 5DS, 6AS, and 7BL, respectively, were perhaps important in defending against FHB by regulating intramolecular transferase activity, GTP binding, or chitinase activity in wheat, but further validation in needed. In addition, a total of five favorable alleles associated with wheat FHB resistance were discovered. These results provide important genes/loci for enhancing FHB resistance in wheat breeding by marker-assisted selection.
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  • 文章类型: Journal Article
    半夏(Thunb。),天南星科的一种多年生草本植物,具有巨大的药用价值和市场需求。2020年8月,严重的叶斑病疫病的爆发导致了巨大的产量损失。有必要分离和鉴定引起P.ternata斑枯病的病原体。
    在这项研究中,我们通过履行科赫的假设来分离和鉴定病原体。收集具有典型斑点疫病症状的疾病样品,并从患病组织中分离病原体。根据其生物学特性和内部转录(rDNA-ITS)和大亚基(LSU)序列的分子分析鉴定了病原体。使用MEGA7软件构建系统发育树,并使用体内接种进行致病性测试。最后,从接种的植物中回收并鉴定病原体。
    根据科赫的假设,我们确定了引起三叶斑枯病的病原体为南瓜孢霉。据我们所知,这是中国首次探索由葫芦枯病引起的斑点病的研究。
    Pinellia ternata (Thunb.), a perennial herbal plant in the Araceae family, has great medicinal value and market demand. In August 2020, an outbreak of severe leaf spot blight disease resulted in a huge yield loss of P. ternata. It is necessary to isolate and identify the pathogens that cause spot blight on P. ternata.
    In this study, we isolated and identified the pathogens by fulfilling Koch\'s postulates. Disease samples with typical spot blight symptoms were collected and pathogens were isolated from the diseased tissues. The pathogen was identified based on its biological characteristics and molecular analysis of internal transcribed (rDNA-ITS) and large subunit (LSU) sequences. Phylogenetic tree were constructed using MEGA7 software and pathogenicity tests were performed using in vivo inoculation. Finally, the pathogen was recovered and identified from the inoculated plants.
    Based on Koch\'s postulates, we identified the pathogen causing spot blight on P. ternata as Stagonosporopsis cucurbitacearum. To our knowledge, this is the first study to explore spot blight on P. ternata caused by S. cucurbitacearum in China.
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  • 文章类型: Journal Article
    未经批准:自2019年武汉冠状病毒病(COVID-19)爆发以来,其在儿童患者中的流行病学和临床特征受到了广泛的关注。然而,临床医生总结和调查SARS-CoV-2在儿童中的合并感染也至关重要。我们回顾了临床表现,实验室发现,合并感染组(CI,n=27)和单一感染组(SI,n=54)。测试样品的多种病原体。发现COVID-19儿童共感染的发生率很高(27/81,33%)。最常见的共感染病原体是肺炎支原体(MP,20/81,25%),其次是病毒(6/81,7%),和细菌(4/81,5%)。临床特征无显著差异,实验室检查,或住院时间在合并感染患者和单抗菌药患者之间观察,白细胞计数仅较低(CI:5.54±0.36vsSI:7.38±0.37,P=0.002),中性粒细胞计数(CI:2.20±0.20vsSI:2.92±0.23,P=.024)和淋巴细胞计数(CI:2.72±0.024vsSI:3.87±0.28,P=.006)。与单抗菌药患者相比,合并感染的患者的胸部影像学显示在更多病例中巩固(CI:29.6%vsSI:11.1%,P=.038),核酸阳性持续时间较短(CI:6.69±0.82vsSI:9.69±0.74,P=.015)。合并感染在COVID-19患儿中相对常见,近1/3合并感染,最常见的原因是MP。共感染并未引起临床表现的明显恶化。
    UNASSIGNED: Since the outbreak of coronavirus disease 2019 (COVID-19) in Wuhan, considerable attention has been paid on its epidemiology and clinical characteristics in children patients. However, it is also crucial for clinicians to summarize and investigate the co-infection of SARS-CoV-2 in children.We retrospectively reviewed the clinical manifestations, laboratory findings, and imaging characteristics of COVID-19 patients in co-infection group (CI, n = 27) and single infection group (SI, n = 54). Samples were tested for multiple pathogens.A high incidence (27/81, 33%) of co-infection in children with COVID-19 was revealed. The most frequent co-infected pathogen was mycoplasma pneumoniae (MP, 20/81, 25%), followed by virus (6/81, 7%), and bacteria (4/81, 5%). No significant difference in clinical characteristics, laboratory examinations, or hospital stay was observed between the patients with co-infections and those with monomicrobial, only lower in white blood cell counts (CI: 5.54 ± 0.36 vs SI: 7.38 ± 0.37, P = .002), neutrophil counts (CI: 2.20 ± 0.20 vs SI: 2.92 ± 0.23, P = .024) and lymphocyte counts (CI: 2.72 ± 0.024 vs SI: 3.87 ± 0.28, P = .006). Compared with the patients with monomicrobial, chest imaging of those with co-infections showed consolidation in more cases (CI: 29.6% vs SI: 11.1%, P = .038) and duration of positive in nucleic acid was shorter (CI: 6.69 ± 0.82 vs SI: 9.69 ± 0.74, P = .015).Co-infection was relatively common in children with COVID-19, almost 1/3 had co-infection, most commonly caused by MP. Co-infection did not cause a significant exacerbation in clinical manifestations.
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  • 文章类型: Journal Article
    我们旨在探讨TLR4(rs4986790)多态性在鼻咽(NP)细菌定植中的作用及其对儿童哮喘发展的影响。对473名2个月大的儿童和213名13个月大的儿童进行了NP拭子的半定量培养。对396名儿童进行TLR4多态性分析。随访儿童从出生到7.5岁,最终结果是医生诊断的哮喘。TLR4基因型之间的关联,细菌定植,和哮喘进行了分析。具有TLR4AG或GG基因型的儿童在2个月大(p=0.009)和13个月大流感嗜血杆菌(p=0.018)时更容易定植。在13个月大的时候定植有流感嗜血杆菌的儿童有明显更高的以后发展为哮喘的风险(p=0.004)。2月龄时卡他莫拉菌或H.流感定植或TLR4基因型Asp299Gly与儿童哮喘的发展无关。TLR4Asp299Gly多态性与儿童粘膜炎莫拉菌和流感嗜血杆菌定植风险增加相关。流感嗜血杆菌在13月龄时的定植与儿童哮喘后期发展的较高风险相关。
    We aimed to explore the role of TLR4 (rs4986790) polymorphism in the nasopharyngeal (NP) bacterial colonization and its consequent impact on the development of childhood asthma. A semi-quantitative culture of NP swabs was performed on 473 children at 2 months of age and on 213 children at 13 months of age. TLR4 polymorphism was analyzed for 396 children. Children were followed from birth to the age of 7.5 years and the final outcome was physician-diagnosed asthma. The associations between TLR4 genotype, bacterial colonization, and asthma were analyzed. Children with TLR4 AG or GG genotype were more often colonized with Moraxella catarrhalis at 2 months of age (p = 0.009) and Haemophilus influenzae at 13 months of age (p = 0.018). Children who were colonized with H. influenzae at 13 months of age had a significantly higher risk of later development of asthma (p = 0.004). M. catarrhalis or H. Influenzae colonization at 2 months of age or TLR4 genotype Asp299Gly were not associated with the development of childhood asthma. TLR4 Asp299Gly polymorphism was associated with an increased risk of colonization of M. catarrhalis and H. influenzae in children. The colonization with H. influenzae at 13 months of age was associated with a higher risk of later development of childhood asthma.
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  • 文章类型: Case Reports
    暂无摘要。
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  • 文章类型: Journal Article
    Understanding the evolutionary path of M. catarrhalis from macrolide-susceptible to macrolide-resistant organism, is important for hindering macrolide resistance from propagation. Multilocus sequence typing (MLST), pulsed-field gel electrophoresis (PFGE) and whole genome SNP typing (WGST), as useful and practical typing tools, have both advantages and disadvantages. We studied the utility of these 3 typing methods, including the level of agreement, consistency and drawbacks, in characterizing M. catarrhalis clones and clonal complexes. We focused on four clonal complexes [CC224, CC363, CC449 (CCN10) and CC446 (CCN08)] and found that PFGE and WGST had a high level of agreement and a proper consistency of the same clone or very closely related clones, while MLST is less discriminatory for different clones. Furthermore, we also established an evolutionary distance cut-off value for \"The same clone\". Moreover, we detected macrolide-resistant M. catarrhalis in CC224, which had previously been considered as a macrolide-susceptible clonal complex. A higher number of isolates belonged to ST215 compared to ST446, implying that ST215 is more likely to be the primary founder. Our study also demonstrated that all the four clonal complexes belong to the M. catarrhalis lineage 1, which is considered to be related to increased virulence potential and serum resistance. We also observed that copB II was highly related to CC449 and LOS type B was mainly confined in CC224. In conclusion, these findings provide further insight into the evolutionary characteristics of M. catarrhalis.
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  • 文章类型: Journal Article
    Infectious bovine keratoconjunctivitis (IBK), also known as pinkeye, is one of the most common eye diseases in cattle. Several pathogens have been associated with IBK cases, however, Moraxella bovis, Moraxella bovoculi, Mycoplasma bovis, Mycoplasma bovoculi and bovine herpesvirus type 1 (BHV-1) are most frequently observed. A multiplex real-time PCR assay using two reactions was developed for the detection and differentiation of these five pathogens. Detection sensitivities of the multiplex assays were compared to singleplex reactions testing for the same targets. Correlation coefficients (R2) of >0.99, and PCR efficiencies between 92 and 106% were demonstrated in all singleplex and multiplex real-time PCR reactions. The limits of detection (LOD) of multiplex assays for Moraxella bovis, Moraxella bovoculi, Mycoplasma bovis, Mycoplasma bovoculi and BHV-1 were 19, 23, 25, 24 and 26 copies per reaction, respectively. No cross amplification was observed for specificity testing of 179 IBK positive clinical samples and 55 non-target clinical samples. Percentage of clinical samples positive for Mycoplasma bovoculi, Moraxella bovoculi, Moraxella bovis, BHV-1 and Mycoplasma bovis were 88.8% (159/179), 75.9% (136/179), 60.3% (108/179), 11.7% (21/179) and 10.0% (18/179), respectively. Moraxella bovis, Moraxella bovoculi and Mycoplasma bovoculi were more prevalent than Mycoplasma bovis and BHV-1 in IBK samples collected from animals in this study population. Our data indicates that the multiplex real-time PCR panel assay is highly sensitive and highly specific for the detection and differentiation of the five major pathogens associated with bovine pinkeye.
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  • 文章类型: Journal Article
    卡他莫拉菌(M.粘膜炎)是一种重要的细菌病原体。然而,由于使用不同的方法和判断标准,其在不同地区的抗生素敏感性模式很难比较。本研究旨在确定从中国两家县级医院收集的卡他莫拉菌的抗菌药物敏感性和β-内酰胺酶活性特征。并参考三个常用的判断标准来表达结果。
    鼻咽拭子取自2015年1-12月在中江县人民医院和佑阳县住院的儿童呼吸道感染患者。从拭子中分离并鉴定了粘膜炎莫拉菌菌株,使用E-test方法或圆盘扩散确定对11种抗菌药物的敏感性。参照欧洲抗菌药物敏感性试验委员会(EUCAST)的标准解释试验结果,临床和实验室标准研究所(CLSI),和英国抗菌药物治疗学会(BSAC)。β-内酰胺酶活性的检测是通过显色头孢菌素硝塞芬测定的。粘附分子的产量分别为7.12和9.58%(中江县,77/1082例;阜阳县,101/1054例,分别)。所有分离株均对阿莫西林-克拉维酸敏感。根据EUCAST,对美罗培南的敏感性为100%;CLSI或BSAC中未列出断点。无论使用何种判断标准,两家医院对磺胺甲恶唑-甲氧苄啶的不敏感率都存在显着差异,来自中江的分离株对来自悠阳的分离株显示出更高的敏感性(费舍尔精确检验,P<0.05)。根据CLSI,对红霉素的总不敏感率为70.8%(中江县,79.2%;阜阳县,64.3%),率达到92.1%(中江县,90.9%;阜阳县,93.1%)在EUCAST或BSAC的基础上。β-内酰胺酶总阳性率为99.4%(177/178例)(中江县,100%,77/77例;阜阳县,99.0%,100/101例)。
    99%的粘膜炎莫拉菌分离物产生β-内酰胺酶。分离株对氨苄西林和红霉素的敏感性差,以及对第三代和第四代头孢菌素和阿莫西林克拉维酸的高度敏感性。注意到不同抗菌药物敏感性判断标准之间存在显着差异。
    Moraxella catarrhalis (M. catarrhalis) is an important bacterial pathogen. However, its antibiotic susceptibility patterns in different areas are difficult to compare because of the use of different methods and judgement criteria. This study aimed to determine antimicrobial susceptibility and β-lactamase activity characteristics of M. catarrhalis isolates collected from two county hospitals in China, and to express the results with reference to three commonly used judgement criteria.
    Nasopharyngeal swabs were obtained from child inpatients with respiratory tract infections at the People\'s Hospital of Zhongjiang County and Youyang County from January to December 2015. M. catarrhalis strains were isolated and identified from the swabs, and susceptibility against 11 antimicrobials was determined using the E-test method or disc diffusion. Test results were interpreted with reference to the standards of the European Committee on Antimicrobial Susceptibility Testing (EUCAST), the Clinical and Laboratory Standards Institute (CLSI), and the British Society for Antimicrobial Chemotherapy (BSAC). Detection of β-lactamase activity was determined by the chromogenic cephalosporin nitrocefin. M. catarrhalis yield rates were 7.12 and 9.58% (Zhongjiang County, 77/1082 cases; Youyang County, 101/1054 cases, respectively). All isolates were susceptible to amoxicillin-clavulanic acid. The susceptibility rate to meropenem was 100% according to EUCAST; no breakpoints were listed in CLSI or BSAC. The non-susceptibility rate to sulfamethoxazole-trimethoprim differed significantly between the two hospitals regardless of the judgemnet criteria used, with isolates from Zhongjiang showing higher susceptibility to those from Youyang (Fisher\'s exact test, P < 0.05). According to CLSI, the total non-susceptibility rate to erythromycin was 70.8% (Zhongjiang County, 79.2%; Youyang County, 64.3%), and the rate reached 92.1% (Zhongjiang County, 90.9%; Youyang County, 93.1%) on the basis of EUCAST or BSAC. The total positive rate of β-lactamase was 99.4% (177/178 cases) (Zhongjiang County, 100%, 77/77 cases; Youyang County, 99.0%, 100/101 cases).
    Ninety nine percent of M. catarrhalis isolates produce β-lactamase. The isolates showed poor susceptibility to ampicillin and erythromycin, and high susceptibility to the third- and fourth-generation cephalosporins and amoxicillin-clavulanic. Significant discrepancies between different antimicrobial susceptibility judgemnet criteria were noted.
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  • 文章类型: Journal Article
    Nasal colonization with bacterial pathogens is associated with risk of invasive respiratory tract infections, but the related information for Chinese healthy children is scarce.
    This cross-sectional study was conducted with healthy children from 6 kindergartens in the Chaoshan region, southern China during 2011-2012. Nasal swabs were examined for five common bacterial pathogens: Streptococcus pneumoniae, Haemophilus influenzae, Haemophilus parainfluenzae, Moraxella catarrhalis, and Staphylococcus aureus.
    Among 1,088 children enrolled, 79.6 % (866) were target-bacterial carriers, of which 34.4 % (298/866) were positive for ≥2 bacteria species. The most common pathogen in the bacterial carriers was M. catarrhalis (76.6 %), followed by S. pneumoniae (26.6 %), S. aureus (21.8 %), H. parainfluenzae (12.7 %), and H. influenzae (2.3 %). Multiple logistic regression analyses showed negative associations between age and the overall or multiple bacterial carriage, and between the father\'s education level and multiple bacterial carriage (all p < 0.05). Age was negatively associated with the carriage of M. catarrhalis and S. pneumoniae, and positively associated with the S. aureus carriage (all p < 0.0001).
    This study shows high nasal carriage of common pathogenic bacteria and coexistence of multiple pathogens in healthy Chaoshan kindergarten children, with M. catarrhalis as the commonest colonizer. Increasing age of children and higher paternal education are associated with lower risk of bacterial carriage. Longitudinal follow-up studies would be helpful for better understanding the infection risk in bacterial pathogen carriers.
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  • 文章类型: Journal Article
    Previous studies indicate that macrolide resistance in Moraxella catarrhalis isolates is less common in adults than in children. However, few studies have investigated M. catarrhalis macrolide resistance mechanisms in adult patients. In this study, 124 M. catarrhalis isolates were collected from adult patients in a Chinese tertiary hospital, between 2010 and 2013, and investigated for antimicrobial resistance. We found that only seven isolates were macrolide resistant and all exhibited high-level macrolide resistance (minimum inhibitory concentrations >256 μg/ml). Multilocus sequence typing (MLST) suggested that M. catarrhalis has a diverse population; in particular, both pulsed-field gel electrophoresis and MLST revealed that all the seven high-level macrolide-resistant M. catarrhalis belonged to different clones. A 934-bp 23S rRNA gene sequencing showed that only nine isolates (including all the seven macrolide-resistant isolates) had mutations within the studied region, and only the seven macrolide-resistant isolates had mutation of A2330T. No other known macrolide-resistance determinant genes (ermA, ermB, mefA, or mefE) were detected. These findings support previous studies in children on M. catarrhalis macrolide-resistant isolates and suggest that the 23S rRNA gene A2330T mutation is responsible for the high M. catarrhalis macrolide resistance. The findings prompted us to successfully develop a simple allele-specific polymerase chain reaction assay for high-level macrolide-resistant 23S rRNA gene A2330T mutation for future clinical and further surveillance use.
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