Department of Biological Sciences, Texas Tech University, Lubbock, TX, 79409-3131, USA.
Transgenic Res. 2020 Jun;29(3):355-367. doi: 10.1007/s11248-020-00196-w. Epub 2020 Apr 23.
Pierce's disease (PD) of grapevine (Vitis vinifera) is caused by the bacterium Xylella fastidiosa and is vectored by xylem sap-sucking insects, whereas Grapevine Red Blotch Virus (GRBV) causes Red Blotch Disease and is transmitted in the laboratory by alfalfa leafhopper Spissistilus festinus. The significance of anthocyanin accumulations in distinct tissues of grapevine by these pathogens is unknown, but vector feeding preferences and olfactory cues from host anthocyanins may be important for these disease etiologies. Phosphate, sugar, and UV light are known to regulate anthocyanin accumulation via miR828 and Trans-Acting Small-interfering locus4 (TAS4), specifically in grape by production of phased TAS4a/b/c small-interfering RNAs that are differentially expressed and target MYBA5/6/7 transcription factor transcripts for post-transcriptional slicing and antisense-mediated silencing. To generate materials that can critically test these genes' functions in PD and GRBV disease symptoms, we produced transgenic grape plants targeting TAS4b and MYBA7 using CRISPR/Cas9 technology. We obtained five MYBA7 lines all with bi-allelic editing events and no off-targets detected at genomic loci with homology to the guide sequence. We obtained two independent edited TAS4b lines; one bi-allelic, the other heterozygous while both had fortuitous evidences of bi-allelic TAS4a off-target editing events at the paralogous locus. No visible anthocyanin accumulation phenotypes were observed in regenerated plants, possibly due to the presence of genetically redundant TAS4c and MYBA5/6 loci or absence of inductive environmental stress conditions. The editing events encompass single base insertions and di/trinucleotide deletions of Vvi-TAS4a/b and Vvi-MYBA7 at expected positions 3 nt upstream from the guideRNA proximal adjacent motifs NGG. We also identified evidences of homologous recombinations of TAS4a with TAS4b at the TAS4a off-target in one of the TAS4b lines, resulting in a chimeric locus with a bi-allelic polymorphism, supporting independent recombination events in transgenic plants associated with apparent high Cas9 activities. The lack of obvious visible pigment phenotypes in edited plants precluded pathogen challenge tests of the role of anthocyanins in host PD and GRBV resistance/tolerance mechanisms. Nonetheless, we demonstrate successful genome-editing of non-coding RNA and MYB transcription factor loci which can serve future characterizations of the functions of TAS4a/b/c and MYBA7 in developmental, physiological, and environmental biotic/abiotic stress response pathways important for value-added nutraceutical synthesis and pathogen responses of winegrape.
葡萄皮尔氏病(PD)由韧皮部杆菌(Xylella fastidiosa)引起,通过木质部汁液吸食昆虫传播,而葡萄红斑病毒(GRBV)引起红斑病,在实验室中由苜蓿叶蝉(Spissistilus festinus)传播。这些病原体在葡萄不同组织中积累花色素苷的意义尚不清楚,但载体的取食偏好和宿主花色素苷的嗅觉线索可能对这些疾病的病因学很重要。已知磷酸盐、糖和紫外线通过 miR828 和 Trans-Acting Small-interfering locus4(TAS4)调节花色素苷的积累,特别是在葡萄中,通过产生相移的 TAS4a/b/c 小干扰 RNA,这些 RNA 差异表达,并针对 MYBA5/6/7 转录因子进行转录后切割和反义介导的沉默。为了生成可在 PD 和 GRBV 疾病症状中对这些基因功能进行严格测试的材料,我们使用 CRISPR/Cas9 技术针对 TAS4b 和 MYBA7 生成了转基因葡萄植物。我们获得了五个 MYBA7 系,所有系均具有双等位基因编辑事件,并且在与引导序列同源的基因组位点上未检测到脱靶。我们获得了两个独立编辑的 TAS4b 系,一个是双等位基因,另一个是杂合子,而这两个系都有同源 TAS4a 脱靶编辑事件的偶然证据,位于旁系同源位点。在再生植物中未观察到明显的花色素苷积累表型,这可能是由于存在遗传冗余的 TAS4c 和 MYBA5/6 基因座,或者缺乏诱导的环境胁迫条件。编辑事件包括在预期位置上游 3nt 处 Vvi-TAS4a/b 和 Vvi-MYBA7 的单个碱基插入和三/二核苷酸缺失,紧邻引导 RNA 近端相邻基序 NGG。我们还在一个 TAS4b 系中鉴定到 TAS4a 与 TAS4b 在 TAS4a 脱靶位点的同源重组证据,导致具有双等位基因多态性的嵌合基因座,支持与明显高 Cas9 活性相关的转基因植物中的独立重组事件。编辑植物中缺乏明显可见的色素表型,排除了对花青素在宿主 PD 和 GRBV 抗性/耐受性机制中作用的病原体挑战测试。尽管如此,我们成功地对非编码 RNA 和 MYB 转录因子基因座进行了基因组编辑,这可以为 TAS4a/b/c 和 MYBA7 在发育、生理和环境生物/非生物胁迫反应途径中的功能提供未来的特征,这些途径对增值营养合成和葡萄病原体反应很重要。
