CN112111470A - 一种R-环结合蛋白GST-His6-1/2×HBD及全基因组R-环的检测方法 - Google Patents
一种R-环结合蛋白GST-His6-1/2×HBD及全基因组R-环的检测方法 Download PDFInfo
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Abstract
本发明提供一种R‑环结合蛋白GST‑His6‑1/2×HBD及全基因组R‑环的检测方法,GST‑His6‑1/2×HBD蛋白能够用于结合和定位R‑环,采用以下步骤制备:重组质粒GST‑His6‑1/2×HBD的构建和提取;将重组质粒转入T7Express lysY/Iq感受态细胞,在2×YT培养基中培养并用IPTG诱导蛋白表达;使用Ni‑NTA beads亲和纯化GST‑His6‑1/2×HBD蛋白。借助其对R‑环结构的特异性结合能力,运用靶向剪切及转座酶技术开发出少量细胞,操作简便,信噪比更高的R‑Loop CUT&TAG,以便更好地绘制内源性R‑环基因组图谱,阐释R‑环在基因组中的功能。
Description
技术领域
本发明属于核酸组学领域,具体涉及一种R-环结合蛋白GST-His6-1/2×HBD及全基因组R-环的检测方法。
背景技术
R-环(R-Loop)是RNA侵入双链DNA所形成的一种特殊的三链核酸结构,包括一条DNA:RNA杂合链和一条单链DNA(single strand DNA,ssDNA)。起初R-环被认为只是转录过程形成的副产物,但是近些年的研究发现R-环在细菌、酵母和哺乳细胞中广泛存在,参与调控整个细胞周期,并在基因表达,染色质结构稳定和DNA损伤修复等过程中起着关键作用。与R-环在转录调控和DNA损伤修复的功能相对应,近年来R-环也被报道与许多疾病相关,比如神经性退行性疾病和癌症。例如,在乳腺癌细胞中,肿瘤抑制因子BRCA1或者BRCA2的突变会造成R-环的积累和DNA损伤的加重,这些R-环直接参与肿瘤的发生,同时也是基因组不稳定的标志。在骨髓增生异常综合征(MDS)的研究中,多种剪切因子的突变也会造成造血干细胞R-环水平的紊乱,从而影响基因组稳定性和细胞功能的正常维持。因此,这些证据表明R-环的异常可能是肿瘤发生的驱动因素之一。
然而,因为R-环功能的多样性,在总量上检测R-环水平的变化并不能阐释R-环在上述生理和病理过程中的作用机制。此外,R-环在转录和复制过程中的调控也显示出“亦正亦邪”的特质,因此近十年来许多研究团队一直在开发基因组水平上R-环的精确定位和定量方法。基于染色质免疫共沉淀技术,Chedin等(2012)首次利用识别DNA:RNA杂交体的S9.6单克隆抗体开发了体外富集R-环的高通量测序技术(DNA:RNA immunoprecipitation withdeep sequencing,DRIP-seq);随后,陈亮等(2015)报道了另外一种基于RNASE H1突变体的R-环检测技术R-CHIP。这些方法虽然将R-环的检测带入了基因组学时代,但是不同检测策略映射出的R-环全基因组图谱存在着很大的差异。此外,这些方法都存在着实验周期长,操作步骤繁琐,信号背景差等缺点,在领域内无法形成一个R-环定位的“金标准”。
发明内容
本发明目的在于提供一种R-环结合蛋白GST-His6-1/2×HBD及全基因组R-环的检测方法,将RNase H1的DNA:RNA杂种结合域HBD进行改良,通过将HBD结构域串联制备特异性识别R-环的重组蛋白GST-His6-1/2×HBD。借助GST-His6-2×HBD对R环结构更强的特异性结合能力,运用最新的靶向剪切及转座酶技术(Cleavage Under Targets andTagmentation,CUT&TAG)进一步开发出少量细胞,操作简便,信噪比更高的R-Loop CUT&TAG,以便更好地绘制内源性R-环基因组图谱,阐释R-环在基因组中的功能。
为实现上述目的,本发明采用以下技术方案:
本发明第一方面提供一种全新的R-环结合蛋白GST-His6-1/2×HBD,所述GST-His6-1/2×HBD蛋白能够用于结合和定位R-环,其采用以下步骤制备:
步骤1:重组质粒GST-His6-1/2×HBD的构建和提取;其中,构建重组质粒GST-His6-1/2×HBD时,质粒结构含有核糖核酸酶RNase H1的DNA:RNA杂交体结合域HBD(HybridBinding Domain),蛋白纯化标签谷胱甘肽S-转移酶(GST-tag)和组氨酸标签(His-tag);
步骤2:将重组质粒GST-His6-1/2×HBD转入T7 Express lysY/Iq感受态细胞,在2×YT培养基中培养并用IPTG诱导蛋白表达;
步骤3:使用Ni-NTA beads亲和纯化GST-His6-1/2×HBD蛋白。
进一步地,在步骤2中,诱导蛋白表达使用0.5mM IPTG,诱导时间为5小时,诱导温度为37℃。
进一步地,所述GST-His6-1/2×HBD蛋白对于R-环的结合能力在体外使用凝胶电泳迁移率分析实验(EMSA)检测。纯化后的GST-His6-1/2×HBD蛋白可以与DNA:RNA杂交体在体外孵育,使用凝胶电泳迁移率分析实验检测核酸与蛋白结合导致的阻滞效应,以此来反映纯化的GST-His6-1/2×HBD蛋白活性以及与R-环的结合能力。
进一步地,在细胞水平结合和定位R-环时采用DRIPc-seq方法,其中免疫沉淀R-环的蛋白为GST-His6-2×HBD。
本发明第二方面提供一种全基因组R-环的检测方法(R-Loop CUT&TAG),采用所述GST-His6-2×HBD蛋白,使用靶向剪切及转座酶技术(CUT&TAG),特异性纯化细胞内R-环。
进一步地,所述靶向剪切及转座酶技术中,所用的pA-Tn5转座酶组装有适配器接头,接头包括:
Tn5MErev(5'-[phos]CTG TCT CTT ATA CAC ATC T-3');
Tn5ME-A(5'-TCG TCG GCA GCG TCA GAT GTG TAT AAG AGA CAG-3');
Tn5ME-B(5'-GTC TCG TGG GCT CGG AGA TGT GTA TAA GAG ACA G-3')。
进一步地,所述靶向剪切及转座酶技术中,R-Loop CUT&TAG测序文库构建之前使用Bst 2.0WarmStart DNA聚合酶完成链置换反应。
进一步地,所述靶向剪切及转座酶技术中,在pA-Tn5转座酶片段化基因组时,反应的缓冲液中添加物包含10%二甲基甲酰胺或者0.85mM ATP,或者两者同时添加。
进一步地,所述靶向剪切及转座酶技术中,可使用单克隆S9.6抗体完成R-LoopCUT&TAG,检测到基因组R-环信号。
进一步地,所述靶向剪切及转座酶技术中在GST-His6-2×HBD蛋白或S9.6抗体孵育过程中,添加RNase A消化后会显著减少富集到的R-环信号。
与现有技术相比,本发明具有以下优点:
(1)本发明使用的GST-His6-1/2×HBD是一种全新的R-环识别因子,解决了之前方法在识别全基因组R-环时由于识别因子特异性问题而产生的争议;
(2)本发明首次提出使用靶向剪切及转座酶技术(CUT&TAG)技术检测全基因组R-环的策略;
(3)R-Loop CUT&TAG耗时短,操作简便,信噪比高,显著提高了R-环检测效率。
附图说明
图1为本发明GST-His6-1/2×HBD重组质粒的构建示意图;
图2为本发明GST-His6-1/2×HBD重组质粒在T7 Express lysY/Iq感受态细胞中,使用原核表达系统设计的蛋白表达与纯化过程;
其中,A图为蛋白表达与纯化流程,B图为蛋白纯化后考马斯亮蓝染色结果;
图3为本发明EMSA实验分析GST-His6-1/2×HBD蛋白对于DNA:RNA杂交体结构的特异性结合能力;
图中,蛋白与核酸结合部分用括号指出,结果显示出GST-His6-1/2×HBD对R-环具有极强的亲和力;
图4为本发明基于已有的DRIPc-seq技术原理,使用GST-His6-2×HBD定位全基因组R-环信号得到的代表性位点示意图;
图中,基因位点示意图显示GST-His6-2×HBD蛋白与S9.6抗体的信号高度一致,阐释了GST-His6-2×HBD蛋白在定位全基因组R-环的可行性;
图5为本发明R-Loop CUT&TAG实验流程示意图;
RNase A可作为对照组添加于抗体结合步骤,以验证该技术在全基因组定位R-环时信号的特异性和真实性;图中,A图表示的是R-Loop CUT&TAG在全基因组定位R-环的实验方法,B图表示的是利用R-环识别因子亲和纯化了基因组R-环后,构建文库用于测序的流程;
图6为本发明R-Loop CUT&TAG在基因组上具有代表性的R-环位点检测到的信号,GST-His6-2×HBD蛋白与S9.6抗体都检测到明显的R-环信号;
图中,在RNase A的消化作用下,R-环的信号显著消失,验证了R-Loop CUT&TAG检测到的R-环的信号特异性和真实性。
具体实施方式
通过以下详细说明结合附图可以进一步理解本发明的特点和优点。所提供的实施例仅是对本发明方法的说明,而不以任何方式限制本发明揭示的其余内容。
本发明中“GST-His6-1/2×HBD”指“GST-His6-1×HBD”或“GST-His6-2×HBD”。
【实施例1】重组质粒GST-His6-1/2×HBD的构建
1.引物的设计合成
根据Marcin Nowotny等(2008)提供了不同物种间RNase H1的高度同源性,从addgene上购得含人源的RNase H1编码序列的ppyCAG-RNASEH1-D210N质粒(addgene#111904),根据质粒信息设计合成特异性引物扩增HBD结构域。在一条引物上加入5个甘氨酸重复序列,表达柔性接头促进串联HBD蛋白表达。引物由上海生工生物工程技术有限公司合成,各引物的序列和编号如下:
(1)HBD基因扩增引物
LP-1:
GCCATATCGAAGGTCGTCATATGATGTTCTATGCCGTGAGGAGGGGC
RP-1:
CTTTGTTAGCAGCCGGTTATCCCCCTCCGCCTCCGCTTGCAGATTTCCT
GACAAAGGC
(2)2×HBD基因扩增引物
LP-2:GTCGTGCATCTGTTGGATATACCATGGGCCATCATCATCAT
RP-2:AGTCAGTCACGATGAATTCCTCCCCCTCCGCCTCC
2.PCR扩增HBD基因与pET16b-His6-HBD重组质粒构建
以ppyCAG-RNASEH1-D210N质粒为模板,使用HBD基因扩增引物与PCR试剂盒(phanta max super-fidelity DNA polymerase,P505-d1,南京诺唯赞生物科技有限公司)特异性扩增HBD基因。用限制性核酸内切酶BamHⅠ和NdeⅠ双酶切pET16b质粒,琼脂糖凝胶电泳后凝胶回收载体片段。利用T5核酸外切酶同源重组修复的原理,将PCR片段与酶切载体以3:1的摩尔比率转化到大肠杆菌DH5α感受态细胞,经过抗性筛选,挑选阳性重组克隆菌种,核苷酸测序验证获得pET16b-His6-HBD重组质粒。
3.GST-His6-1/2×HBD重组质粒构建
以pET16b-His6-HBD重组质粒为模板,使用2XHBD基因扩增引物特异性扩增His6-HBD基因。用限制性核酸内切酶BamHⅠ和EcoRⅠ双酶切pGEX-2T质粒,琼脂糖凝胶电泳后凝胶回收载体片段。采取步骤2同样的同源重组技术,筛选获得GST-His6-1/2×HBD重组质粒,质粒结构示意图见图1。
【实施例2】GST-His6-1/2×HBD蛋白表达与纯化
1.GST-His6-1/2×HBD蛋白表达
将GST-His6-1/2×HBD重组质粒转化到T7 Express lysY/Iq感受态细胞,经过抗性筛选,挑选单克隆菌种培养在含100μg/mL氨苄青霉素钠的2×YT培养基,细菌培养条件设置为37℃,转速200rpm。当细菌的OD600达到0.6时,加入0.5mM IPTG诱导蛋白表达。培养5小时后离心收集细菌颗粒,除去多余的培养基,加入pH7.5的裂解HEX缓冲液(组分包括20mMHEPES,0.8M氯化钠,10%甘油,0.2%Triton X-100,1X蛋白酶抑制剂)。缓冲液与细菌充分混匀后使用细胞破碎仪进行高压破碎,4℃,800psi条件下破碎5分钟,然后高速离心收集上清,此时上清包含有可溶性的GST-His6-1/2×HBD蛋白。
2.GST-His6-1/2×HBD蛋白纯化
依照Ni-NTA Beads(SA004010,常州天地人和生物科技有限公司)说明书亲和纯化GST-His6-1/2×HBD蛋白。在上一步获得的上清中加入1/20体积的Ni-NTA Beads,4℃孵育过夜。在蛋白纯化柱中,依次加入含有20mM咪唑和100mM咪唑的HEX缓冲液,洗去非目的蛋白,直至洗涤液中无蛋白组分洗出,最终使用含250mM咪唑的HEX缓冲液纯化目的蛋白。纯化的目的蛋白在4℃环境中透析过夜,多次透析去除咪唑后,使用超滤管浓缩。使用SDS-PAGE分析GST-His6-1/2×HBD蛋白纯度,然后用BCA蛋白定量试剂盒(PA115-01,北京天根生化科技有限公司)检测蛋白浓度。GST-His6-1/2×HBD蛋白纯化流程与纯化结果见图2。
【实施例3】GST-His6-1/2×HBD蛋白特异性识别R-环结构
(1)凝胶电泳迁移率分析实验(EMSA)检测不同浓度的GST-His6-1/2×HBD蛋白与DNA:RNA杂交体的结合能力,反应条件和体系如下:
用移液器将上述组分混匀,在PCR热循环仪上进行以下反应:25℃孵育30分钟
(2)将步骤(1)的样品加入到6%TBE-PAGE凝胶中进行电泳,电泳缓冲液为0.5×TBE,电泳电压设置为60V,电泳时间为60分钟。
(3)使用GE公司的Typhoon9500扫描凝胶,根据核酸在凝胶内的阻滞现象验证GST-His6-1/2×HBD蛋白能特异性结合DNA:RNA杂交体,具体结果见图3。
【实施例4】基于DRIPc-seq,GST-His6-2×HBD蛋白定位基因组R-环根据Chedin等(2019)设计的DRIPc-seq方案
(1)基因组分离与片段化:消化收集1×107数量的HEK293T细胞,加入20%SDS与蛋白酶K在37℃水浴条件下过夜消化细胞,然后利用酚氯仿法抽提细胞基因组。加入BsrGI,EcoRI,HindIII,SspI和XbaI这五种限制性内切酶后,37℃过夜消化基因组,使用酚氯仿抽提回收片段化的基因组DNA。
(2)R-环分离与纯化:加入GST-His6-2×HBD蛋白在4℃条件下孵育14~17h,利用特异性结合GST标签的磁珠分离纯化HBD蛋白及其结合的R-环结构。经过蛋白酶K消化后,使用酚氯仿抽提获得纯化的R-环。
(3)基于RNA的建库:用DNASE I消化上一步获得的R-环中的DNA,以此得到R-环结构中的RNA链,再通过逆转录反应合成cDNA,经第二链补齐形成双链DNA,然后在DNA两端添加接头标签,建库并在Nova-seq上进行高通量测序。基因组具有代表性的R-环位点见图4。
【实施例5】一种基因组学定位R-环方法:R-Loop CUT&TAG
以HEK293T细胞为例
(1)5×105数量的细胞经过accutase消化后收集,接下来使用PH7.5的洗涤缓冲液(组分包括20mM HEPES,150mM氯化钠,0.5mM亚精胺,1×蛋白酶抑制剂)洗涤2次。细胞中加入10μl活化的刀豆球蛋白A包被磁珠,室温孵育10分钟后洗脱磁珠,完成细胞的固定和穿孔过程。
(2)接下来孵育GST-His6-2×HBD蛋白或者S9.6抗体,以识别细胞内特定的R-环结构。根据相应的蛋白依次孵育anti-GST或者anti-His-tag抗体或者兔抗鼠IgG抗体,以及对应的二抗,实现R-环信号的富集。
(3)使用pH7.5的dig-wash缓冲液(组分包括20mM HEPES,300mM氯化钠,0.5mM亚精胺,1×蛋白酶抑制剂,0.05%毛地黄皂苷)洗涤三次以去除未结合的蛋白。加入带有适配接头的pA-Tn5转座酶复合物,在pH8.5的片段化缓冲液(组分包括10mM TAPS,10mM氯化镁,10%二甲基甲酰胺,0.85mM ATP)中室温孵育1小时完成片段化反应。
(4)然后添加2.25μl 0.5M乙二胺四乙酸,2.75μl 10%SDS和0.5μg蛋白酶K,在55℃条件下反应30分钟终止片段化反应。片段化产物经DNA磁珠回收后使用Bst2.0WarmStart DNA聚合酶完成链置换反应。
(5)最后使用Q5高保真混合体系完成文库构建后用于高通量测序,实验流程设计见图5,检测到的R-环信号见图6。
Claims (10)
1.一种R-环结合蛋白GST-His6-1/2×HBD,其特征在于:所述GST-His6-1/2×HBD蛋白能够用于结合和定位R-环,其采用以下步骤制备:
步骤1:重组质粒GST-His6-1/2×HBD的构建和提取;
其中,构建重组质粒GST-His6-1/2×HBD时,质粒结构含有核糖核酸酶RNase H1的DNA:RNA杂交体结合域HBD(Hybrid Binding Domain),蛋白纯化标签谷胱甘肽S-转移酶(GST-tag)和组氨酸标签(His-tag);
步骤2:将步骤1得到的重组质粒GST-His6-1/2×HBD转入T7 Express lysY/Iq感受态细胞,在2×YT培养基中培养并用IPTG诱导蛋白表达;
步骤3:使用Ni-NTA beads亲和纯化步骤2的GST-His6-1/2×HBD蛋白。
2.如权利要求1所述的R-环结合蛋白GST-His6-1/2×HBD,其特征在于:在步骤2中,诱导蛋白表达使用0.5mM IPTG,诱导时间为5小时,诱导温度为37℃。
3.如权利要求1或2所述的R-环结合蛋白GST-His6-1/2×HBD,其特征在于:所述GST-His6-1/2×HBD蛋白对于R-环的结合能力在体外使用凝胶电泳迁移率分析实验(EMSA)检测。
4.如权利要求1所述的R-环结合蛋白GST-His6-1/2×HBD,其特征在于:在细胞水平结合和定位R-环应用DRIPc-seq方法,其中免疫沉淀R-环的蛋白为GST-His6-2×HBD。
5.一种全基因组R-环的检测方法,其特征在于:采用权利要求1所述的GST-His6-2×HBD蛋白,使用靶向剪切及转座酶技术,特异性纯化细胞内R-环。
6.如权利要求5所述的全基因组R-环的检测方法,其特征在于:所述靶向剪切及转座酶技术中,所用的pA-Tn5转座酶组装有适配器接头,接头包括:
Tn5MErev:5'-[phos]CTG TCT CTT ATA CAC ATC T-3';
Tn5ME-A:5'-TCG TCG GCA GCG TCA GAT GTG TAT AAG AGA CAG-3';
Tn5ME-B:5'-GTC TCG TGG GCT CGG AGA TGT GTA TAA GAG ACA G-3'。
7.如权利要求5或6所述的全基因组R-环的检测方法,其特征在于:所述靶向剪切及转座酶技术中,R-Loop CUT&TAG测序文库构建之前使用Bst 2.0WarmStart DNA聚合酶完成链置换反应。
8.如权利要求7所述的全基因组R-环的检测方法,其特征在于:所述靶向剪切及转座酶技术中,在pA-Tn5转座酶片段化基因组时,反应的缓冲液中添加物包含终浓度为10%二甲基甲酰胺或者0.85mM ATP,或者两者同时添加。
9.如权利要求8所述的全基因组R-环的检测方法,其特征在于:所述靶向剪切及转座酶技术中,可使用单克隆S9.6抗体完成R-Loop CUT&TAG,检测到基因组R-环信号。
10.如权利要求8或9所述的全基因组R-环的检测方法,其特征在于:所述靶向剪切及转座酶技术中,在GST-His6-2×HBD蛋白或S9.6抗体孵育过程中,添加RNase A消化能够显著减少富集到的R-环信号。
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