Division of Biology and Howard Hughes Medical Institute, California Institute of Technology, Pasadena, CA, USA.
PLoS One. 2013;8(1):e54971. doi: 10.1371/journal.pone.0054971. Epub 2013 Jan 28.
The identity of each neuron is determined by the expression of a distinct group of genes comprising its terminal gene battery. The regulatory sequences that control the expression of such terminal gene batteries in individual neurons is largely unknown. The existence of a complete genome sequence for C. elegans and draft genomes of other nematodes let us use comparative genomics to identify regulatory sequences directing expression in the DVA interneuron.
METHODOLOGY/PRINCIPAL FINDINGS: Using phylogenetic comparisons of multiple Caenorhabditis species, we identified conserved non-coding sequences in 3 of 10 genes (fax-1, nmr-1, and twk-16) that direct expression of reporter transgenes in DVA and other neurons. The conserved region and flanking sequences in an 85-bp intronic region of the twk-16 gene directs highly restricted expression in DVA. Mutagenesis of this 85 bp region shows that it has at least four regions. The central 53 bp region contains a 29 bp region that represses expression and a 24 bp region that drives broad neuronal expression. Two short flanking regions restrict expression of the twk-16 gene to DVA. A shared GA-rich motif was identified in three of these genes but had opposite effects on expression when mutated in the nmr-1 and twk-16 DVA regulatory elements.
CONCLUSIONS/SIGNIFICANCE: We identified by multi-species conservation regulatory regions within three genes that direct expression in the DVA neuron. We identified four contiguous regions of sequence of the twk-16 gene enhancer with positive and negative effects on expression, which combined to restrict expression to the DVA neuron. For this neuron a single binding site may thus not achieve sufficient specificity for cell specific expression. One of the positive elements, an 8-bp sequence required for expression was identified in silico by sequence comparisons of seven nematode species, demonstrating the potential resolution of expanded multi-species phylogenetic comparisons.
每个神经元的身份由其末端基因库中独特的一组基因决定。控制个体神经元中这些末端基因库表达的调节序列在很大程度上是未知的。由于秀丽隐杆线虫的完整基因组序列和其他线虫的草图基因组的存在,我们可以使用比较基因组学来识别指导 DVA 中间神经元表达的调节序列。
方法/主要发现:通过对多个秀丽隐杆线虫物种的系统发育比较,我们在 10 个基因中的 3 个(fax-1、nmr-1 和 twk-16)中鉴定出了指导 DVA 和其他神经元中报告基因表达的保守非编码序列。twk-16 基因内含子 85 个碱基对的保守区域和侧翼序列指导 DVA 中的高度受限表达。该 85 个碱基对区域的突变显示它至少有四个区域。中央的 53 个碱基对区域包含一个 29 个碱基对的区域,该区域抑制表达,一个 24 个碱基对的区域驱动广泛的神经元表达。两个短的侧翼区域将 twk-16 基因的表达限制在 DVA 中。在这三个基因中,我们发现了三个共享的富含 GA 的基序,但在 nmr-1 和 twk-16 的 DVA 调节元件中突变时,它们对表达的影响是相反的。
结论/意义:我们通过多物种保守性鉴定出了三个基因内的调节区域,这些区域指导 DVA 神经元的表达。我们鉴定出 twk-16 基因增强子的四个连续序列区域,这些区域对表达具有正、负效应,它们共同将表达限制在 DVA 神经元中。因此,对于这个神经元来说,一个单一的结合位点可能不足以实现细胞特异性表达的足够特异性。一个正元件,一个表达所需的 8 个碱基对序列,通过对 7 种线虫物种的序列比较在计算机上鉴定出来,证明了扩展的多物种系统发育比较的潜在分辨率。