PCR‐RFLP

PCR - RFLP
  • 文章类型: Journal Article
    背景:尿道下裂仍然是影响男性外生殖器的常见先天性异常,其特点是起源不明确,治疗方法复杂。这项研究旨在调查与尿道下裂相关的危险因素,并探讨其与DICER1rs3742330变异的遗传联系。
    方法:本研究包括两组:105名尿道下裂男性儿童和111名健康男性儿童作为配对对照。对所有患者和对照组进行详细的病史和体格检查。PCR限制性片段长度多态性用于鉴定DICER1rs3742330变体,分析基因型分布和等位基因频率。Logistic回归分析估计尿道下裂的危险因素。
    结果:尿道下裂组的平均年龄为4.56±2.50岁。观察到的最常见的尿道下裂类型是60名儿童(57.14%)的前部型。宫内生长受限,高龄产妇,和妊娠期高血压被确定为尿道下裂的显著危险因素(分别为p=.011,p=.016和p=.041).关于基因研究,病例组和对照组的DICER1rs3742330变异体的基因型和等位基因频率均无显著差异.
    结论:DICER1基因的rs3742330变异与阿尔及利亚人群尿道下裂病例无关联。然而,多变量逻辑回归分析确定早产,低出生体重,宫内生长受限,高龄产妇,妊娠期糖尿病,和农村居住地是尿道下裂最重要的独立预测因子。
    BACKGROUND: Hypospadias continues to be a prevalent congenital anomaly affecting the male external genitalia, characterized by an unclear origin and complex treatment approaches. This study aimed to investigate the risk factors associated with hypospadias and explore its genetic link with the DICER1 rs3742330 variant.
    METHODS: The study involved two groups: 105 male children with hypospadias and 111 healthy male children as matched controls. Detailed history and physical examinations were conducted for all patients and controls. PCR-restriction fragment length polymorphism was utilized to identify the DICER1 rs3742330 variant, analyzing genotype distribution and allele frequency. Logistic regression analysis estimated the risk factors for hypospadias.
    RESULTS: The mean age in the hypospadias group was 4.56 ± 2.50 years. The most prevalent type of hypospadias observed was the anterior type in 60 children (57.14%). Intrauterine growth restriction, advanced maternal age, and gestational hypertension were identified as significant risk factors for hypospadias (p = .011, p = .016, and p = .041, respectively). Regarding the genetic study, no significant difference was found in both genotype and allele frequencies of the DICER1 rs3742330 variant between case and control groups.
    CONCLUSIONS: The rs3742330 variant in the DICER1 gene showed no association with hypospadias cases in the Algerian population. However, multivariate logistic regression analysis identified preterm birth, low birth weight, intrauterine growth restriction, advanced maternal age, gestational diabetes, and rural residence as the most significant independent predictors for hypospadias.
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  • 文章类型: Journal Article
    转录终止因子中的停止增益突变(rs715966442;BTA11:1,02,463,944核苷酸位置),RNA聚合酶I(TTF1)基因导致荷斯坦弗里斯(HF)牛流产。已开发并验证了基于PCR限制性片段长度多态性(PCR-RFLP)的遗传测试,以筛选HF牛的TTF1突变位点。使用该方案在80个HF和HF杂种中筛选了突变基因座,揭示了两只动物是突变TTF1等位基因的携带者。采用的测试具有成本效益,快速,准确,可用作筛选HF牛群中TTF1突变携带者的有效工具。
    A stop-gain mutation (rs715966442; BTA11: 1,02,463,944 nucleotide position) in transcription termination factor, RNA polymerase I (TTF1) gene causes abortion in Holstein Friesian (HF) cattle. A PCR-restriction fragment length polymorphism (PCR-RFLP)-based genetic test has been developed and validated to screen the TTF1 mutation locus in HF cattle. The mutation locus was screened in 80 HF and HF crossbreds using the protocol, which revealed two animals as carriers of the mutant TTF1 allele. The test employed is cost-effective, rapid and precise and can be utilized as an effective tool for the screening of TTF1 mutation carriers in HF cattle population.
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  • 文章类型: Journal Article
    锡林郭勒本土羊品种的肌肉在中国很有名,并且该人群中的FecB基因型仍未表征。在这项研究中,通过焦磷酸测序研究FecB基因座中的SNP,并产生了优化的PCR-RFLP技术来鉴定SNP。此外,使用TaqMan实时PCR和品种保守引物和SNP特异性探针优化了FecB中高通量SNP鉴定的有效技术。通过使用新型的TaqMan实时PCR方法对锡林郭勒本地绵羊品种的肌肉中的FecB基因座进行基因分型,我们的研究为将来基于特定基因鉴定锡林郭勒羊肉和使用标记辅助选择策略对锡林郭勒绵羊进行多产性育种奠定了基础。
    The muscle from Xilingol indigenous sheep breeds are famous in China, and the FecB genotype in this population remains uncharacterized. In this study, SNPs in the FecB locus were investigated by pyrosequencing, and an optimized PCR-RFLP technique was generated to identify SNPs. In addition, an efficient technique for high-throughput identification of SNPs in FecB was optimized using TaqMan real-time PCR and breed-conservative primers and SNP-specific probes. By genotyping the FecB locus in the muscle of Xilingol indigenous sheep breeds using a novel TaqMan real-time PCR assay, our study has generated the groundwork for the authentication of Xilingol mutton based on the specific gene and the prolificacy-oriented breeding of Xilingol sheep using marker-assisted selection strategies in the future.
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  • 文章类型: Journal Article
    Thunnini,或者金枪鱼,包括许多具有不同商业价值的物种。市场上主要的生金枪鱼产品是生鱼片,使用的物种很难通过常规的形态学分析来鉴定。本研究扩增了用于制备生鱼片黄鳍金枪鱼(Thunnusalbacares)的4种主要金枪鱼的细胞色素b基因(Cytb),南部蓝鳍金枪鱼(Thunnusmaccoyii),大眼金枪鱼(Thunnusobesus),和大西洋蓝鳍金枪鱼(Thunnusthynnus)-和4种通常被错误标记为金枪鱼生鱼片-长鳍金枪鱼(Thunnusalalunga)的成分的物种,金枪鱼(Katsuwonuspelamis),条纹马林鱼(Tetrapturusaudax),和旗鱼(剑兰)。用5种限制酶-Eco147I消化聚合酶链反应(PCR)扩增子,如果我,MboI,XagI,和HindII-以获得上述原始金枪鱼物种和通常错误标记的物种的特征限制图。建立了使用PCR限制性片段长度多态性(PCR-RFLP)的鉴定方法,并使用39个商业金枪鱼刺身样品进行了验证,这证实了该方法提供的结果与通过经典测序获得的结果一致。PCR-RFLP比经典测序有几个优点,比如简单,速度和准确性。该技术可以支持对生金枪鱼和生鱼片的物种鉴定。
    The Thunnini, or tuna, comprise many species with very different commercial values. The principal raw tuna product on the market is sashimi, for which the species used is difficult to identify through conventional morphological analysis. The present study amplified the cytochrome b gene (Cytb) of 4 major tuna species used for preparing sashimi-yellowfin tuna (Thunnus albacares), southern bluefin tuna (Thunnus maccoyii), bigeye tuna (Thunnus obesus), and Atlantic bluefin tuna (Thunnus thynnus)-and 4 species commonly mislabeled as components of tuna sashimi-albacore tuna (Thunnus alalunga), skipjack tuna (Katsuwonus pelamis), striped marlin (Tetrapturus audax), and swordfish (Xiphias gladius). Polymerase chain reaction (PCR) amplicons were digested with 5 restriction enzymes-Eco147 I, Hinf I, Mbo I, Xag I, and Hind II-to obtain characteristic restriction maps of the above-mentioned raw tuna species and the commonly mislabeled species. An identification method using PCR restriction fragment length polymorphism (PCR-RFLP) was established and validated using 39 commercial tuna sashimi samples, which verified that this method provides results consistent with those obtained by classical sequencing. PCR-RFLP has several advantages over classical sequencing, such as simplicity, speed and accuracy. This technique could support species identification for raw tuna and sashimi.
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  • 文章类型: Journal Article
    果蝇果蝇是研究后生生物学几个方面的模型生物。大部分工作是在成年果蝇中进行的,包括实验室和野外标本,但是果蝇幼虫最近成为更好地了解动物生理学的有价值的模型,发展,或宿主-微生物相互作用。虽然成年果蝇可以根据形态特征轻松地分配给给定的果蝇物种,这种视觉识别在幼虫阶段更加复杂。这可以解释为什么关注幼虫的研究数量有限,尤其是场衍生样本。这里,我们开发了一种聚合酶链反应-限制性片段长度多态性(PCR-RFLP)测定法,该测定法可在幼虫期将黑腹果蝇与其他与生态相关的果蝇区分开。方法,靶向细胞色素氧化酶I(COI)基因,使用来自不同地理区域的七个D.melanogaster种群以及六个果蝇物种的实验室幼虫进行了验证。我们在自然环境中进一步验证了这种PCR-RFLP测定,通过识别在法国两个地方收集的野生幼虫。值得注意的是,在所有与黑腹D.melanogaster物种匹配的PCR-RFLP图谱中,100%被正确识别,如COI测序所证实。总之,我们的工作提供了一个快速,简单,和精确的分子工具,从野外采集的幼虫中鉴定黑腹。
    The fruit fly Drosophila melanogaster is a model organism to study several aspects of metazoan biology. Most of the work has been conducted in adult fruit flies, including laboratory and field-derived specimens, but Drosophila melanogaster larvae recently became a valuable model to better understand animal physiology, development, or host-microbe interactions. While adult flies can be easily assigned to a given Drosophila species based on morphological characteristics, such visual identification is more intricate at the larval stage. This could explain the limited number of studies focusing on larvae, especially field-derived samples. Here, we developed a polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) assay that discriminates D. melanogaster from other ecologically relevant Drosophila species at the larval stage. The method, which targets the cytochrome oxidase I (COI) gene, was validated using laboratory-derived larvae from seven D. melanogaster populations originating from different geographic areas as well as six Drosophila species. We further validated this PCR-RFLP assay in a natural context, by identifying wild larvae collected in two locations in France. Notably, among all PCR-RFLP profiles that matched the D. melanogaster species, 100% were correctly identified, as confirmed by COI sequencing. In summary, our work provides a rapid, simple, and accurate molecular tool to identify D. melanogaster from field-collected larvae.
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  • 文章类型: Journal Article
    Competition theory states that multiple species should not be able to occupy the same niche indefinitely. Morphologically, similar species are expected to be ecologically alike and exhibit little niche differentiation, which makes it difficult to explain the co-occurrence of cryptic species. Here, we investigated interspecific niche differentiation within a complex of cryptic bumblebee species that co-occur extensively in the United Kingdom. We compared the interspecific variation along different niche dimensions, to determine how they partition a niche to avoid competitive exclusion. We studied the species B. cryptarum, B. lucorum, and B. magnus at a single location in the northwest of Scotland throughout the flight season. Using mitochondrial DNA for species identification, we investigated differences in phenology, response to weather variables and forage use. We also estimated niche region and niche overlap between different castes of the three species. Our results show varying levels of niche partitioning between the bumblebee species along three niche dimensions. The species had contrasting phenologies: The phenology of B. magnus was delayed relative to the other two species, while B. cryptarum had a relatively extended phenology, with workers and males more common than B. lucorum early and late in the season. We found divergent thermal specialisation: In contrast to B. cryptarum and B. magnus, B. lucorum worker activity was skewed toward warmer, sunnier conditions, leading to interspecific temporal variation. Furthermore, the three species differentially exploited the available forage plants: In particular, unlike the other two species, B. magnus fed predominantly on species of heather. The results suggest that ecological divergence in different niche dimensions and spatio-temporal heterogeneity in the environment may contribute to the persistence of cryptic species in sympatry. Furthermore, our study suggests that cryptic species provide distinct and unique ecosystem services, demonstrating that morphological similarity does not necessarily equate to ecological equivalence.
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