A deletion at the polled PC locus alone is not sufficient to cause a polled phenotype in cattle

Hennig, Sadie L.; Owen, Joseph R.; Lin, Jason; McNabb, Bret R.; Eenennaam, Alison L. Van; Murray, James D.

doi:10.1038/s41598-022-06118-6

Cited by 6 publications

(7 citation statements)

References 39 publications

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“…This disagrees with a previous study that suggested a HAND1 binding site was altered by the 10‐bp deletion of P C (Nguyen et al, 2018). The knock‐out of a genomic region including these 10 bases resulting bovine fetuses were horned (Hennig et al, 2022). The overall evidence, therefore, suggests that P C does not interrupt an enhancer.…”

Section: Resultsmentioning

confidence: 99%

“…Nguyen et al (2018) mapped predicted bovine regulatory elements to the POLLED locus and found that the 10‐bp deletion of P C may interrupt a transcription factor binding site. However, when gene editing was used to knock out the 10‐bp deletion, the bovine fetuses remained horned (Hennig et al, 2022). This indicates that the 10‐bp deletion of P C is not responsible for the polled phenotype and that the 212‐bp duplication is likely to be the cause.…”

Section: Introductionmentioning

confidence: 99%

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Topologically associating domains in the POLLED region are the same for Angus‐ and Brahman‐specific Hi‐C reads from F1 hybrid fetal tissue

et al. 2023

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Horns are a form of headgear carried by Bovidae, including cattle, sheep, goats, and yak, and have welfare and economic implications for production systems (Simon et al., 2022). Hornless (polled) animals occur naturally in some domesticated Bovidae and are usually preferentially selected. Four dominant genetic variants are known to be associated with polled in cattle and are located within a 300-kb region on chromosome 1 (BTA1) 1 (Aldersey et al., 2020). The Celtic variant (P C ) consists of a 212-bp duplication and a 10-bp deletion (Medugorac et al., 2012). The Friesian variant (P F ) is an ~80-kb tandem duplication (Medugorac et al., 2012). The Mongolian variant (P M ) is a complex 219-bp duplication insertion with an additional 6-bp deletion and 7-bp insertion

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Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Topologically associating domains in the POLLED region are the same for Angus‐ and Brahman‐specific Hi‐C reads from F1 hybrid fetal tissue

et al. 2023

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“…Mosaicism is a common problem observed when using genome editing reagents in developing embryos. Our previous work reported an inverse correlation between mosaicism rate and timing of injections hours post insemination (hpi), with the lowest mosaicism rates being seen in embryos edited 6 hpi 28 . Interestingly, we saw this same trend in the work presented here.…”

Section: Discussionmentioning

confidence: 97%

LincRNA#1 knockout alone does not affect polled phenotype in cattle heterozygous for the celtic POLLED allele

Hennig

McNabb

Trott

et al. 2022

Sci Rep

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A long intergenic non-coding RNA (lincRNA#1) is overexpressed in the horn bud region of polled (hornless) bovine fetuses, suggesting a potential role in horn bud suppression. Genome editing was used to test whether the absence of this sequence was associated with the horned phenotype. Two gRNAs with high mutation efficiencies targeting the 5′ and the 3′ regions flanking the lincRNA#1 sequence were co-injected with Cas9 as ribonucleoprotein complexes into bovine zygotes (n = 121) 6 h post insemination. Of the resulting blastocysts (n = 31), 84% had the expected 3.7 kb deletion; of these embryos with the 3.7 kb deletions, 88% were biallelic knockouts. Thirty-nine presumptive edited 7-day blastocysts were transferred to 13 synchronized recipient cows resulting in ten pregnancies, five with embryos heterozygous for the dominant PCPOLLED allele at the POLLED locus, and five with the recessive pp genotype. Eight (80%) of the resulting fetuses were biallelic lincRNA#1 knockouts, with the remaining two being mosaic. RT-qPCR analysis was used to confirm the absence of lincRNA#1 expression in knockout fetuses. Phenotypic and histological analysis of the genotypically (PCp) POLLED, lincRNA#1 knockout fetuses revealed similar morphology to non-edited, control polled fetuses, indicating the absence of lincRNA#1 alone does not result in a horned phenotype.

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“…An issue with this strategy is that it has been well documented that microinjection of gene editing reagents into fish and mammalian zygotes results in progeny having more than two alleles (mosaicism), and often the frequency of these alleles is disproportionate and can vary across different tissues analyzed (Lamas-Toranzo et al 2019;Mehravar et al 2019;Hennig et al 2020Hennig et al , 2022. Mosaicism is typically the result of one or more of the following variables: (i) timing of nuclease injection (premeiotic, one cell, two cell), (ii) nuclease activity at intended target site, (iii) class of nuclease (Zinc Finger, Meganuclease, TALEN, Cas9, CPF1), (iv) reagents delivered (DNA, mRNA, protein), concentration, and associated half-life, and (v) target site accessibility in different cell types.…”

Section: Scaled Gene Modificationmentioning

confidence: 99%

Technical considerations towards commercialization of porcine respiratory and reproductive syndrome (PRRS) virus resistant pigs

Cigan

Knap²

2022

CABI Agric Biosci

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The selection and introduction of disease resistance genes in livestock not only provide health benefits to animals but opportunities for breeders and farmers to meet the growing demand for high-quality meat and milk while reducing agriculture’s footprint on the environment. As traditional methods of classical breeding and selection for trait improvement are slow, recent progress in several areas of biology including (a) understanding host–pathogen interactions, (b) inexpensive and rapid DNA sequencing, and (c) robust gene editing like CRISPR-Cas provide geneticists tools to accelerate discovery and deployment of disease resistance alleles in livestock. Using these advances, the introduction of resistance genes into commercially relevant germplasm requires access to genetically superior livestock, an infrastructure for scalable allele deployment, freedom to operate, global regulatory approvals, and acceptance of gene edited livestock by producers and consumers. Importantly, academic researchers have recently discovered that modification of the CD163 gene in pigs can confer resistance to the virus that causes porcine reproductive and respiratory syndrome (PRRS). While this achievement represents a major step towards solving an important disease in livestock, to realize the positive impact on animal health while benefiting the pork industry and consumers, it is necessary to introduce this recessive disease resistance allele into commercial breeding populations. Rather than backcrossing the resistance gene from a few non-commercial founders, as a global supplier of high genetic merit livestock genetics, Genus plc and its pig division PIC (Pig Improvement Company) with Genus R&D have mobilized advances in reproductive biology, gene editing, DNA sequencing, and bioinformatics to simultaneously generate and introduce a single modified CD163 allele across four genetically diverse porcine lines of commercial importance that prevents PRRS virus (PRRSV) infection. This report focuses on technical aspects for a scaled gene editing program to consider for rapid and efficient generation and advancement of a small population of non-transgenic founder pigs for commercial breeding. This high genetic merit herd containing a PRRS disease resistance allele will provide important benefits to animal health and food chain value once approved for commercial sale and export.

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A deletion at the polled PC locus alone is not sufficient to cause a polled phenotype in cattle

Cited by 6 publications

References 39 publications

Topologically associating domains in the POLLED region are the same for Angus‐ and Brahman‐specific Hi‐C reads from F1 hybrid fetal tissue

Topologically associating domains in the POLLED region are the same for Angus‐ and Brahman‐specific Hi‐C reads from F1 hybrid fetal tissue

LincRNA#1 knockout alone does not affect polled phenotype in cattle heterozygous for the celtic POLLED allele

Technical considerations towards commercialization of porcine respiratory and reproductive syndrome (PRRS) virus resistant pigs

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