High-throughput CRISPR Vector Construction and Characterization of DNA Modifications by Generation of Tomato Hairy Roots

Jacobs, Thomas B.; Martin, Gregory B.

doi:10.3791/53843

Cited by 28 publications

(29 citation statements)

References 25 publications

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“…Due to genetic redundancy for MYBA5/6/7 and TAS4a/b/c loci, it remains to be determined whether the events characterized here will have visible phenotypes impacting anthocyanin pigmentation and/or PD resistance/tolerance. Future experiments can employ multiple guide constructs (Jacobs and Martin 2016) to target all MYBA and TAS4 family members, and to target the sole Vvi-MIR828 locus at locations upstream or downstream of the mature miR828 in the hairpin structure to generate leaky dominant-negative alleles predicted to alter DICER processing efficiency. Our initial test construct for Vvi-MIR828 aimed to create null alleles by targeting the mature miR828 duplex per se but we failed to recover any regenerants, consistent with a speculated essential function of MIR828.…”

Section: Discussionmentioning

confidence: 99%

CRISPR/Cas9-mediated targeted mutagenesis of TAS4 and MYBA7 loci in grapevine rootstock 101-14

Sunitha

Rock

2020

Transgenic Res

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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 TransActing 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

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Section: Discussionmentioning

confidence: 99%

CRISPR/Cas9-mediated targeted mutagenesis of TAS4 and MYBA7 loci in grapevine rootstock 101-14

Sunitha

Rock

2020

Transgenic Res

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“…Three gRNAs were selected to specifically target each of the LRR-XII gene family members as well as a control phytoene desaturase (PDS), as a knockout would result in obvious photobleaching (Liu et al, 2002; Supplemental Table S1). The 165 gRNAs were synthesized, pooled, and cloned into a Cas9 binary vector using DNA assembly (Jacobs and Martin, 2016). Sequencing of 105 Escherichia coli clones indicated that there was no obvious gRNA bias from the library preparation (Supplemental Table S2).…”

Section: Targeting the Lrr-rlk Subfamily XII Gene Family In Tomatomentioning

confidence: 99%

“…For each gene, the target sequences and their coordinates were extracted, and a custom Perl script was used to select the top three nonoverlapping gRNAs for each gene. Oligonucleotides were designed with the GN 19 sequences plus 20-nucleotide overlapping regions of the MtU6 promoter and scaffold for DNA assembly with NEBuilder HiFi DNA Assembly Master Mix (New England Biolabs), as described previously (Jacobs and Martin, 2016). Oligonucleotides were synthesized and pooled in equimolar amounts by Integrated DNA Technologies.…”

Section: Designing Grna Targets and Library Cloningmentioning

confidence: 99%

Generation of a Collection of Mutant Tomato Lines Using Pooled CRISPR Libraries

et al. 2017

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The high efficiency of clustered regularly interspaced short palindromic repeats (CRISPR)-mediated mutagenesis in plants enables the development of high-throughput mutagenesis strategies. By transforming pooled CRISPR libraries into tomato (), collections of mutant lines were generated with minimal transformation attempts and in a relatively short period of time. Identification of the targeted gene(s) was easily determined by sequencing the incorporated guide RNA(s) in the primary transgenic events. From a single transformation with a CRISPR library targeting the immunity-associated leucine-rich repeat subfamily XII genes, heritable mutations were recovered in 15 of the 54 genes targeted. To increase throughput, a second CRISPR library was made containing three guide RNAs per construct to target 18 putative transporter genes. This resulted in stable mutations in 15 of the 18 targeted genes, with some primary transgenic plants having as many as five mutated genes. Furthermore, the redundancy in this collection of plants allowed for the association of aberrant T0 phenotypes with the underlying targeted genes. Plants with mutations in a homolog of an Arabidopsis () boron efflux transporter displayed boron deficiency phenotypes. The strategy described here provides a technically simple yet high-throughput approach for generating a collection of lines with targeted mutations and should be applicable to any plant transformation system.

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“…Overexpressing transgenic lines were generated with EVE under control of the 35S cauliflower promoter. For generation of CRISPR/Cas9 EVE mutant plants, a guide RNA (gRNA) targeting EVE was selected from http://aspendb.uga.edu/ (56), and cloned as previously described (57). Constructs were transferred into Agrobacterium and transformation of the hybrid (P. tremula × alba) poplar genotype 717-1B4 was performed (58).…”

Section: Methodsmentioning

confidence: 99%

The uncharacterized geneEVEcontributes to vessel element dimensions inPopulus

Ribeiro

Conde

Balmant

et al. 2020

Proc. Natl. Acad. Sci. U.S.A.

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The radiation of angiosperms led to the emergence of the vast majority of today's plant species and all our major food crops. Their extraordinary diversification occurred in conjunction with the evolution of a more efficient vascular system for the transport of water, composed of vessel elements. The physical dimensions of these water-conducting specialized cells have played a critical role in angiosperm evolution; they determine resistance to water flow, influence photosynthesis rate, and contribute to plant stature. However, the genetic factors that determine their dimensions are unclear. Here we show that a previously uncharacterized gene, ENLARGED VESSEL ELEMENT (EVE), contributes to the dimensions of vessel elements in Populus, impacting hydraulic conductivity. Our data suggest that EVE is localized in the plasma membrane and is involved in potassium uptake of differentiating xylem cells during vessel development. In plants, EVE first emerged in streptophyte algae, but expanded dramatically among vessel-containing angiosperms. The phylogeny, structure and composition of EVE indicates that it may have been involved in an ancient horizontal gene-transfer event.vessel | xylem | EVE | vessel dimension | phycodnavirus

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High-throughput CRISPR Vector Construction and Characterization of DNA Modifications by Generation of Tomato Hairy Roots

Cited by 28 publications

References 25 publications

CRISPR/Cas9-mediated targeted mutagenesis of TAS4 and MYBA7 loci in grapevine rootstock 101-14

CRISPR/Cas9-mediated targeted mutagenesis of TAS4 and MYBA7 loci in grapevine rootstock 101-14

Generation of a Collection of Mutant Tomato Lines Using Pooled CRISPR Libraries

The uncharacterized geneEVEcontributes to vessel element dimensions inPopulus

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