Loss of the Na+/K+ cation pump CATP-1 suppresses nekl-associated molting defects.

IF 2.1 3区 生物学 Q3 GENETICS & HEREDITY
Shaonil Binti, Phil T Edeen, David S Fay
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Abstract

The conserved Caenorhabditis elegans protein kinases NEKL-2 and NEKL-3 regulate membrane trafficking and are required for larval molting. Through a forward genetic screen we identified a mutation in catp-1 as a suppressor of molting defects in synthetically lethal nekl-2; nekl-3 double mutants. catp-1 encodes a membrane-associated P4-type ATPase involved in Na+-K+ exchange. A previous study found that wild-type worms exposed to the nicotinic agonist dimethylphenylpiperazinium (DMPP) exhibited larval arrest and molting-associated defects, which were suppressed by inhibition of catp-1. By testing a spectrum catp-1 alleles, we found that resistance to DMPP toxicity and the suppression of nekl defects did not strongly correlate, suggesting key differences in the mechanism of catp-1-mediated suppression. Through whole genome sequencing of additional nekl-2; nekl-3 suppressor strains, we identified two additional coding-altering mutations in catp-1. However, neither mutation, when introduced into nekl-2; nekl-3 mutants using CRISPR, was sufficient to elicit robust suppression of molting defects, suggesting the involvement of other loci. Endogenously tagged CATP-1 was primarily expressed in epidermal cells within punctate structures located near the apical plasma membrane, consistent with a role in regulating cellular processes within the epidermis. Based on previous studies, we tested the hypothesis that catp-1 inhibition induces entry into the pre-dauer L2d stage, potentially accounting for the ability of catp-1 mutants to suppress nekl molting defects. However, we found no evidence that loss of catp-1 leads to entry into L2d. As such, loss of catp-1 may suppress nekl-associated and DMPP-induced defects by altering electrochemical gradients within membrane-bound compartments.

Na+/K+阳离子泵CATP-1的缺失可抑制nekl相关的蜕皮缺陷。
保守的秀丽隐杆线虫蛋白激酶 NEKL-2 和 NEKL-3 可调节膜运输,是幼虫蜕皮所必需的。通过正向遗传筛选,我们发现 catp-1 突变抑制了合成致死的 nekl-2;nekl-3 双突变体的蜕皮缺陷。catp-1 编码一种参与 Na+-K+ 交换的膜相关 P4 型 ATP 酶。之前的一项研究发现,野生型蠕虫暴露于烟碱激动剂二甲苯基哌嗪(DMPP)后会出现幼虫停育和蜕皮相关缺陷,而抑制 catp-1 则可抑制这些缺陷。通过测试一系列 catp-1 等位基因,我们发现对 DMPP 毒性的抗性和对 nekl 缺陷的抑制并不密切相关,这表明 catp-1 介导的抑制机制存在关键差异。通过对额外的 nekl-2;nekl-3 抑制株进行全基因组测序,我们在 catp-1 中发现了两个额外的编码改变突变。然而,当使用CRISPR技术将这两个突变导入nekl-2;nekl-3突变体时,它们都不足以对蜕皮缺陷产生强有力的抑制作用,这表明有其他基因位点的参与。内源标记的 CATP-1 主要在表皮细胞中位于顶端质膜附近的点状结构中表达,这与 CATP-1 在表皮细胞过程中的调控作用一致。基于之前的研究,我们测试了 catp-1 抑制诱导进入前道尔 L2d 阶段的假设,这可能是 catp-1 突变体抑制 nekl 蜕化缺陷的原因。然而,我们没有发现任何证据表明 catp-1 的缺失会导致进入 L2d 阶段。因此,catp-1的缺失可能是通过改变膜结合区室中的电化学梯度来抑制nekl相关缺陷和DMPP诱导的缺陷。
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来源期刊
G3: Genes|Genomes|Genetics
G3: Genes|Genomes|Genetics GENETICS & HEREDITY-
CiteScore
5.10
自引率
3.80%
发文量
305
审稿时长
3-8 weeks
期刊介绍: G3: Genes, Genomes, Genetics provides a forum for the publication of high‐quality foundational research, particularly research that generates useful genetic and genomic information such as genome maps, single gene studies, genome‐wide association and QTL studies, as well as genome reports, mutant screens, and advances in methods and technology. The Editorial Board of G3 believes that rapid dissemination of these data is the necessary foundation for analysis that leads to mechanistic insights. G3, published by the Genetics Society of America, meets the critical and growing need of the genetics community for rapid review and publication of important results in all areas of genetics. G3 offers the opportunity to publish the puzzling finding or to present unpublished results that may not have been submitted for review and publication due to a perceived lack of a potential high-impact finding. G3 has earned the DOAJ Seal, which is a mark of certification for open access journals, awarded by DOAJ to journals that achieve a high level of openness, adhere to Best Practice and high publishing standards.
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