VC2 调节蚕豆中的基线维卡因含量

bioRxiv Pub Date : 2024-08-08 DOI:10.1101/2024.08.06.606773
S. Ugwuanyi, M. Makhoul, A. Golicz, C. Obermeier, Rod J. Snowdon
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引用次数: 0

摘要

蚕豆(Vicia faba)是一种珍贵的豆类作物,因其营养成分高而受到全球的青睐。然而,种子中的黄豆碱和卷心菜碱(v-c)含量会降低蚕豆蛋白的营养质量,并可能诱发葡萄糖-6-磷酸脱氢酶缺乏症患者的蚕豆中毒。最近有报道称,编码双功能核黄素蛋白的 VC1 基因负责启动蚕豆的生物合成途径。在低 v-c 栽培品种中,该基因的 2 bp 插入导致功能缺失,但该突变仅部分消除了 v-c 的生物合成,表明还有其他基因的参与。在这里,我们证明了一个新的蚕豆核黄素基因 VC2 是造成蚕豆中 v-c 含量残留的原因。VC2 与 VC1 的功能域几乎相同,具有 GTP 环醇酶 II 活性,可催化 GTP 转化为生物合成途径中的中间分子。基因表达分析表明,VC2 对性状的影响较小,约占核黄素基因总转录本的 5-10%,这与低 v-c 栽培品种的基线含量显著相关。我们的结果表明,由于 VC2 的活性,在 VC1 中携带 2 bp 失活插入片段的栽培品种仍有残余的 v-c 水平。此外,我们还发现 VC1 有多个等位基因,并表现出拷贝数变异,这使得分子标记的开发变得更加复杂。相反,VC2 中的单核苷酸多态性为蚕豆育种中的标记辅助选择提供了可靠的替代方法。总之,我们的研究阐明了 v-c 生物合成的复杂遗传调控,并为促进消除蚕豆中的 v-c 提供了宝贵的见解。
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VC2 regulates baseline vicine content in faba bean
Faba bean (Vicia faba) is a valuable legume crop desired globally for its high nutritional composition. However, the seed vicine and convicine (v-c) content reduces the nutritional quality of faba bean protein and can induce favism in individuals with glucose-6-phosphate dehydrogenase deficiency. Recently, VC1 gene, encoding a bi-functional riboflavin protein, was reported to be responsible for initiating the biosynthetic pathway in V. faba. In low v-c cultivars, a 2 bp insertion in this gene results in a loss of function, but the mutation only partially eliminates v-c biosynthesis, indicating the involvement of other genes. Here, we demonstrate that a novel V. faba riboflavin gene, VC2, is responsible for the residual v-c contents in faba bean. VC2 shares nearly identical functional domains with VC1 and has GTP cyclohydrolase II activity, catalyzing the conversion of GTP into an intermediate molecule in the biosynthetic pathway. Gene expression analysis reveals that VC2 contributes a minor effect to the trait, accounting for approximately 5-10% of total riboflavin gene transcripts which significantly correlates with the baseline contents in low v-c cultivars. Our results illustrate that cultivars carrying the 2 bp inactivating insertion in VC1 still have residual v-c levels due to VC2 activity. Furthermore, we find that VC1 has multiple alleles and exhibits copy number variations, complicating molecular marker development. Conversely, single nucleotide polymorphisms within VC2 provide a reliable alternative for marker-assisted selection in faba bean breeding. In conclusion, our study elucidates the complex genetic regulation of v-c biosynthesis and provides valuable insights to facilitate its elimination in faba bean.
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