Machwe Amrita, Xiao Liren, Orren David K
Graduate Center for Toxicology, College of Medicine, University of Kentucky, Lexington, KY 40536-0305, USA.
BMC Mol Biol. 2006 Feb 17;7:6. doi: 10.1186/1471-2199-7-6.
The cancer-prone and accelerated aging disease Werner syndrome is caused by loss of function of the WRN gene product that possesses ATPase, 3' to 5' helicase and 3' to 5' exonuclease activities. Although WRN has been most prominently suggested to function in telomere maintenance, resolution of replication blockage and/or recombinational repair, its exact role in DNA metabolism remains unclear. WRN is the only human RecQ family member to possess both helicase and exonuclease activity, but the mechanistic relationship between these activities is unknown. In this study, model single-stranded and 3' overhang DNA substrates of varying length and structure were used to examine potential coordination between the ATPase/helicase and exonuclease activities of WRN.
Our results show that WRN can not only bind to but also catalyze the 3' to 5' degradation of single-stranded and 3' overhang DNA substrates, structures that were previously thought to be refractory to WRN exonuclease activity. The length of the single-stranded regions in these structures is a critical parameter in determining both the binding affinity and the level of exonuclease activity of WRN. Most importantly, specific nucleotide cofactors dramatically stimulate WRN exonuclease activity on these substrates, with conditions that permit ATP hydrolysis not only resulting in enhanced exonuclease activity but also altering its length dependence on these structures. Parallel experiments show that a deletion mutant containing only the WRN exonuclease domain lacks both this DNA length and nucleotide cofactor dependence, demonstrating that the interaction of the ATPase/helicase domain of WRN with the DNA substrate has a profound influence on exonuclease activity.
Our results indicate that, under conditions that permit ATP hydrolysis, there is a dynamic and cooperative relationship between the distinct ATPase/helicase and exonuclease domains of WRN with regard to their orientation on DNA. Based on these results, models are proposed for the coordinated, unidirectional 3' to 5' movement of the helicase and exonuclease domains of WRN on DNA that should be informative for elucidating its function in genome maintenance.
癌症易感性和加速衰老疾病沃纳综合征是由WRN基因产物功能丧失引起的,该产物具有ATP酶、3'至5'解旋酶和3'至5'核酸外切酶活性。尽管WRN最显著地被认为在端粒维持、复制阻滞的解决和/或重组修复中发挥作用,但其在DNA代谢中的确切作用仍不清楚。WRN是人类RecQ家族中唯一同时具有解旋酶和核酸外切酶活性的成员,但其这些活性之间的机制关系尚不清楚。在本研究中,使用不同长度和结构的模型单链和3'突出端DNA底物来研究WRN的ATP酶/解旋酶和核酸外切酶活性之间的潜在协同作用。
我们的结果表明,WRN不仅可以结合单链和3'突出端DNA底物,还可以催化其3'至5'降解,而这些结构以前被认为对WRN核酸外切酶活性具有抗性。这些结构中单链区域的长度是决定WRN结合亲和力和核酸外切酶活性水平的关键参数。最重要的是,特定的核苷酸辅因子显著刺激WRN对这些底物的核酸外切酶活性,允许ATP水解的条件不仅导致核酸外切酶活性增强,还改变了其对这些结构的长度依赖性。平行实验表明,仅包含WRN核酸外切酶结构域的缺失突变体既缺乏这种DNA长度依赖性,也缺乏核苷酸辅因子依赖性,这表明WRN的ATP酶/解旋酶结构域与DNA底物的相互作用对核酸外切酶活性有深远影响。
我们的结果表明,在允许ATP水解的条件下,WRN不同的ATP酶/解旋酶和核酸外切酶结构域在DNA上的方向之间存在动态协同关系。基于这些结果,提出了WRN的解旋酶和核酸外切酶结构域在DNA上协调、单向3'至5'移动的模型,这对于阐明其在基因组维持中的功能应该具有指导意义。
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