Molecular identification of DNA barcoding of Leguminous toxic species and quantitative analysis by ELISA kits

IF 1.7 4区 生物学 Q4 BIOTECHNOLOGY & APPLIED MICROBIOLOGY
Jie Wang, Shuangyu Wang, Fenglin Sun, Chang Liu, Jinquan Zhao, Hongwei Yu, Xiaojing Lv, Ze Liu, Shuhua Bu, Weisen Yu
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Abstract

Some edible Leguminous are toxic when raw, and the Chinese are particularly fond of beans, so Leguminous poisoning is very common in China. Rapid and accurate identification of poisoned species and determination of their toxic components would better assist physicians in treating patients. However, traditional morphology-based identification methods possess many limitations. DNA barcoding technique is a new species identification technique developed in recent years, which is expected to make up for the shortcomings of traditional morphological identification. In this study, a comprehensive evaluation system based on DNA barcoding and ELISA kits was attempted. A total of 30 Leguminous toxic plants were collected, involving 9 genera and 10 species. We used simulated gastric fluid (SGF) to simulate the human gastric environment. Three markers (rbcL, trnH-psbA, and ITS) were amplified and sequenced for all untreated and 15 mock-digested samples. The validity of DNA barcoding for species identification was assessed using the Basic Local Alignment Search Tool (BLAST) method and the tree construction method. The levels of three toxic components (saponin, phytoagglutin and trasylol) were determined in all samples using ELISA kits. The amplification success rate of all three regions was high (rbcL 96.67%, trnH-psbA 100%, and ITS 100%), but the sequencing of the trnH-psbA region was less satisfactory (66.67%), and SGF had a significant impact on the sequencing of the ITS region (After 40 min of SGF treatment, the sequencing success rate decreased by 46.67%). The samples from different species and origins contained different levels of toxic components, and the levels of all three substances decreased significantly after undergoing SGF digestion. After 1 h of SGF treatment, the saponin content decreased to 0–8.60% in untreated content (PHA decreased to 8.62–36.88%, trasylol decreased to 4.70–47.06%). The current results suggest that DNA barcoding has great potential for rapid identification of Leguminous poisoning in clinical settings. Toxins are probably not detectable in the patient for longer periods of poisoning. We recommend DNA barcoding technology as a first step for rapid screening and combined with toxin analysis for clinical diagnosis.

Abstract Image

豆科有毒物种 DNA 条形码的分子鉴定和酶联免疫吸附试剂盒的定量分析
一些可食用的豆科植物生吃有毒,而中国人又特别喜欢吃豆子,因此豆科植物中毒在中国非常常见。快速准确地鉴定中毒种类并确定其毒性成分,能更好地帮助医生治疗病人。然而,传统的基于形态学的鉴定方法存在很多局限性。DNA条形码技术是近年来发展起来的一种新的物种鉴定技术,有望弥补传统形态鉴定的不足。本研究尝试建立基于 DNA 条形编码和 ELISA 试剂盒的综合评价体系。共采集了 30 种豆科有毒植物,涉及 9 属 10 种。我们使用模拟胃液(SGF)来模拟人类胃部环境。对所有未处理样本和 15 个模拟消化样本的三个标记(rbcL、trnH-psbA 和 ITS)进行了扩增和测序。使用基本局部比对搜索工具(BLAST)方法和树构建方法评估了DNA条形码在物种鉴定中的有效性。使用酶联免疫吸附试剂盒测定了所有样本中三种有毒成分(皂苷、植物凝集素和三苯酚)的含量。三个区域的扩增成功率都很高(rbcL 96.67%、trnH-psbA 100%、ITS 100%),但 trnH-psbA 区域的测序结果不太理想(66.67%),SGF 对 ITS 区域的测序结果有明显影响(SGF 处理 40 分钟后,测序成功率下降了 46.67%)。不同物种和产地的样品含有不同含量的有毒成分,经过 SGF 消解后,这三种物质的含量都明显下降。经过 1 小时的 SGF 处理后,皂苷含量下降到未处理含量的 0-8.60%(PHA 下降到 8.62-36.88%,三苯酚下降到 4.70-47.06%)。目前的研究结果表明,DNA 条形码技术在临床上快速鉴定豆科植物中毒方面具有很大的潜力。中毒时间较长的患者体内可能检测不到毒素。我们建议将 DNA 条形码技术作为快速筛查的第一步,并结合毒素分析进行临床诊断。
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来源期刊
Plant Biotechnology Reports
Plant Biotechnology Reports 生物-生物工程与应用微生物
CiteScore
4.10
自引率
4.20%
发文量
72
审稿时长
>12 weeks
期刊介绍: Plant Biotechnology Reports publishes original, peer-reviewed articles dealing with all aspects of fundamental and applied research in the field of plant biotechnology, which includes molecular biology, genetics, biochemistry, cell and tissue culture, production of secondary metabolites, metabolic engineering, genomics, proteomics, and metabolomics. Plant Biotechnology Reports emphasizes studies on plants indigenous to the Asia-Pacific region and studies related to commercialization of plant biotechnology. Plant Biotechnology Reports does not exclude studies on lower plants including algae and cyanobacteria if studies are carried out within the aspects described above.
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