CN105950640B - 以海洋细菌为来源获取的κ-卡拉胶酶基因及重组酶制备方法 - Google Patents
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Abstract
本发明涉及分子生物学和基因工程领域,具体来讲涉及一种以海洋细菌为来源编码获取Κ‑卡拉胶酶基因的及重组酶制备方法。本发明包括如下步骤:一、PCR法获得海洋细菌中κ‑卡拉胶酶基因的全长序列;二、以海洋细菌为来源基因κ‑卡拉胶酶基因的重组表达质粒和重组菌株的构建;三、利用重组表达菌株表达重组κ‑卡拉胶酶;四、重组酶的活性检测。本发明通过一种新的、高效、准确的途径,以海洋细菌为来源获得的κ‑卡拉胶酶基因应用于大肠杆菌工程菌株的构建,并实现具有活性重组酶的异源表达,为实现工业化生产卡拉胶酶提供基础;通过本发明中的以海洋细菌为来源获得的κ‑卡拉胶酶基因,与已知κ‑卡拉胶酶序列相似性最高为44%。
Description
技术领域:
本发明涉及分子生物学和基因工程领域,具体来讲涉及一种以海洋细菌为来源编码获取Κ-卡拉胶酶基因的及重组酶制备方法。
背景技术:
卡拉胶酶(Carrageenase)是一种海藻多糖水解酶,可降解卡拉胶的β-1,4糖苷键,生成系列偶数的卡拉胶寡糖。根据识别底物特异性,可将卡拉胶降解酶分为以下三种:κ-卡拉胶酶(EC 3.2.1.83)、ι-卡拉胶酶(EC 3.2.1.157)和λ-卡拉胶酶(EC 3.2.1.162)。κ-卡拉胶酶(κ-Carrageenase)属于糖苷水解酶GH16家族,该家族成员还包括昆布多糖酶、β-琼胶酶、内切β-1,3-1,4-葡聚糖酶、内切β-牛乳糖苷酶和木葡聚糖转移酶等,它们有共同的保守核心催化区域E[ILV]D[IVAF][VILMF(0,1)]E序列。ι-卡拉胶酶(ι-Carrageenase)属于糖苷水解酶GH 82家族。具有DFGX3DGX6AX3A的糖苷酶保守区域。λ-卡拉胶酶(λ-Carrageenase)既不属于κ-卡拉胶酶的GH16,也不属于ι-卡拉胶酶的GH82,是一类新型的糖苷水解酶家族。
卡拉胶酶主要来源海洋微生物,也有部分来源海洋软体动物。已在假单胞菌属(Pseudomonas)、别单胞菌属(Alteromonas)、噬纤维菌属(Cellulophaga)、弧菌属(Vibrio)、黄杆菌属(Flavobacteriales)、浮霉菌属(Planctomycetales)、毛螺旋菌科(Lachnospiraceae)、紫红球菌目(Puniceicoccales)等微生物中发现了不同类型卡拉胶酶。卡拉胶酶在这些微生物体内的存在方式具有多样性。例如λ-卡拉胶酶仅存在某些特定的微生物,有些微生物体内同时具有多种类型的卡拉胶降解酶,例如Pseudoalteromonascarrageenovora能同时分泌κ-、λ-和ι-卡拉胶酶,而Alteromonas carrageenovora和Zobellia galactanovorans能同时分泌κ-和ι-卡拉胶降解酶。
目前关于卡拉胶酶的研究主要包括生化方面和分子生物学方面。前者主要集中在卡拉胶酶高产菌株的选育、发酵剂产酶条件的优化、酶学性质研究、降解机制及产物鉴定;后者主要集中编码卡拉胶酶基因的克隆、序列分析、重组表达、酶的纯化及酶学性质研究等。虽然大量卡拉胶酶高产菌株被发现,并对其产酶发酵条件和酶学特性进行了大量研究,但目前卡拉胶酶无法满足规模化酶解法制备卡拉胶寡糖的需求。酶解法制备卡拉胶寡糖研究领域中存在:产酶量和酶活力普遍较低,无法达到规模化生产的要求;野生菌株培养体系复杂,海洋来源需要大量的NaCl,为后续卡拉胶寡糖的纯化增加产本产酶条件不稳定;容易出现菌种退化,无法连续生产等问题。采用分子生物学技术从编码卡拉胶酶的功能基因入手,通过基因克隆、序列分析、重组表达、表达特性及构效关系方面的研究是解决上述困难的有效方法之一,而获得优良的编码卡拉胶酶的基因是进行上述工作的基础。
现有的分子生物学技术多数还是采用文库构建等传统方法获取卡拉胶酶基因,但文库构建工作费时费力,需要通过大量筛选获得阳性克隆,进而通过亚克隆等环节才能获得完整基因。伴随着高通量测序技术的发展,海量基因组被解析并释放基因组数据,如何借助这些基因组数据服务于卡拉胶酶基因的挖掘是亟待解决的问题。如果有一种方法能在比较基因组学分析的基础上,借助于传统同源克隆的原理而从基因组中通过一次PCR方法获得完整目的基因,则可以免除上述文库构建的繁琐工作,从而实现目的基因的高效获得。
发明内容:
本发明的目的⑴是提供一种从产卡拉胶酶的菌株中通过一次PCR方法直接获得完整目的基因的方法,建立了一种新的、高效、准确的途径,并将获得的κ-卡拉胶酶基因应用于大肠杆菌工程菌株的构建,并实现具有活性重组酶的异源表达,为实现工业化生产卡拉胶酶提供基础。
本发明的目的⑵是利用该方法克隆获得一个全新海洋细菌来源κ-卡拉胶酶基因。
本发明的目的⑶是利用限制性内切酶,将克隆获得的卡拉胶酶基因连接到原核表达载体pET-28a(+)中,构建卡拉胶酶基因的表达载体pET-28a(+)-Cly-κ-car,通过转化技术将表达载体转入到大肠杆菌(BL21),构建工程菌株,最终获得能产活性重组卡拉胶酶的BL21-Cly-κ-CAR工程菌株。
本发明的技术方案包括如下步骤:
一、PCR法获得海洋细菌C.lytica M9中κ-卡拉胶酶基因的全长序列
⑴根据海洋细菌C.lytica M9(菌种保藏号:CGMCC No:10829)中16s RNA序列构建系统进化树,找到与目的菌株最相近且具有全基因组数据的参考菌株(Cellulophagalytica DSM 7489,基因组数据信息NC_015167);
⑵根据基因组注释信息和NCBI中blast程序验证之后,找到参考菌株(C.lyticaDSM7489)基因组中编码κ-卡拉胶酶的基因Celly_2915编号(gi|325284916:3333332-3334777蛋白序列ADY30732),同时确定该参考菌株中编码κ-卡拉胶酶的相邻上游基因Celly_2914编号(gi|325284916:3332347-3333021蛋白序列ADY30731)和下游基因Celly_2916编号(gi|325284916:3335359-3336312蛋白序列ADY30733)及分别对应的核苷酸和氨基酸序列;
⑶根据相邻上下游基因(Celly_2914和Celly_2916)的氨基酸序列通过BlocκMaκer在线软件程序进行比对和寻找保守核心区域,其中,Celly_2914的核心保守序列为:QGSINPM和Celly_2916的核心保守序列为:SGLGEPNE;
⑷根据Celly_2914基因的核心保守序列采用CODEHOP软件设计正向引物,
正向引物为:TCTTGCTTCGCTACCAGCTC;
根据根据Celly_2916基因的核心保守序列采用CODEHOP软件设计反向引物,
反向引物为:TTTGGCTCTCCCAAACCAGA;
⑸以目的菌株C.lytica M9基因组为模板,利用步骤⑷中所述的引物经一步PCR方法获得一种全新的海洋细菌为来源,含有编码完整κ-卡拉胶酶基因的原始编码序列,其核苷酸序列为Seq ID.NO.1,该基因DNA序列全长1488bp,编码495个氨基酸,含有45个氨基酸的信号肽序列。κ-卡拉胶酶的氨基酸序列为Seq ID.NO.2,该酶属于糖苷水解酶GH16家族。
二、海洋细菌C.lytica M9来源基因κ-卡拉胶酶基因的重组表达质粒和重组菌株的构建
将上一步骤获得的κ-卡拉胶酶基因克隆到原核表达载体pET-28a(+)中,构建重组表达质粒。首先基于获得的κ-卡拉胶酶基因的全长序列(采用软件预测ORF中的信号肽区域),设计获取目的基因成熟肽部分的上下游引物:
上游引物Cly-κ-Car-F:CCCGAATTCCAAACATCTAATCCGAATGATAATT
下游引物Cly-κ-Car-R:GGCTCGAGCTATTGAATAAGCAGTTGTTTTG;
采用含有原始编码序列的质粒pMD-18T-原始编码序列模板,通过PCR方法获得目的基因成熟肽部分序列。采用限制性内切酶EcoR I和Xho I双酶切PCR产物,胶回收酶切之后的片段,跟同样经过EcoR I和Xho I双酶切的质粒pET-28a(+)链接,按照CaCl2转化法转化到大肠杆菌TOP10中,卡那霉素抗性筛选阳性克隆。采用质粒抽提试剂盒提取阳性克隆质粒,通过测序和EcoR I和Xho I双酶切鉴定,获得目的基因的(Cly-κ-car)重组表达质粒pET-28a(+)-Cly-κ-car,将该质粒进一步转化到大肠杆菌BL21中,构建重组表达工程菌株BL21-Cly-κ-CAR。
三、利用重组表达菌株BL21-Cly-κ-CAR表达重组κ-卡拉胶酶
将活化好的1ml重组表达菌株BL21-Cly-κ-CAR转接到100ml含有20pg/ml卡那霉素的LB液体培养基中,LB液体培养基为1000ml去离子水中胰蛋白胨10g、酵母提取物5g、NaCl10g,用5mol/LNaOH调pH至7.0。37℃振荡培养(培养条件37℃,转速150r/min)至OD600达到0.6-0.8,将培养液温度降至18℃度左右,此时加入终浓度为0.l mM的IPTG进行诱导表达,诱导条件为18℃,转速100r/min,培养24h,离心收集菌体,将50ml菌体重悬于20ml海洋细菌C.lytica M9发酵培养基中(C.lytica M9发酵培养基:每100ml陈海水中卡拉胶0.1%、蛋白胨0.5%、FeSO4.7H2O 0.002%),在冰上进行超声波破碎处理,低温离心收集上清,上清液即为粗酶液,SDS-PAGE检测上清中目的基因的表达量。
四、重组Cly-κ-CAR酶的活性检测。
本发明的有益效果为,本发明通过一种新的、高效、准确的途径,以海洋细菌为来源获得的κ-卡拉胶酶基因应用于大肠杆菌工程菌株的构建,并实现具有活性重组酶的异源表达,为实现工业化生产卡拉胶酶提供基础;通过本发明中的以海洋细菌为来源获得的κ-卡拉胶酶基因,与已知κ-卡拉胶酶序列相似性最高为44%(NCBI:WP_013991622,Zobelliagalactanivorans),经重组表达之后,最高酶活可达到100-120U/ml。
附图说明:
图1为重组κ-卡拉胶酶的SDS-PAGE电泳图,其中:C代表对照,1、2、3分别代表诱导6h、8h、24h,M代表蛋白分子量;
图2为重组κ-卡拉胶酶的酶谱图,其中:4代表降解条带,M代表蛋白分子量。
具体实施方式:
现结合说明书附图和具体实施方式进一步说明本发明。
实施例1:一步PCR法获得海洋细菌C.lytica M9中κ-卡拉胶酶基因的全长序列
⑴根据海洋细菌C.lytica M9中16s RNA序列构建系统进化树,找到与目的菌株最相近且具有全基因组数据的参考菌株(Cellulophaga lytica DSM 7489,基因组数据信息NC_015167),其核苷酸序列与Seq ID.NO:1所示序列一致;
⑵根据基因组注释信息找到参考菌株(C.lytica DSM 7489)基因组中编码κ-卡拉胶酶的基因Celly_2915编号(gi|325284916:3333332-3334777蛋白序列ADY30732),同时确定该参考菌株中编码κ-卡拉胶酶的相邻上游基因Celly_2914编号(gi|325284916:3332347-3333021蛋白序列ADY30731)和下游基因Celly_2916编号(gi|325284916:3335359-3336312蛋白序列ADY30733)及分别对应的核苷酸和氨基酸序列;
⑶根据相邻上下游基因(Celly_2914和Celly_2916)的氨基酸序列通过BlocκMaκer在线软件程序进行比对和寻找保守核心区域(Celly_2914的核心保守序列:QGSINPM和Celly_2916的核心保守序列:SGLGEPNE);
⑷根据Celly_2914基因的核心保守序列QGSINPM,采用CODEHOP软件设计正向引物(正向引物:TCTTGCTTCGCTACCAGCTC),根据根据Celly_2916基因的核心保守序列SGLGEPNE,采用CODEHOP软件设计反向引物(反向引物:TTTGGCTCTCCCAAACCAGA);
⑸以目的菌株C.lytica M9基因组为模板,利用本发明所述的方法包括如下步骤⑷中所述的简并引物经一步PCR方法获得卡拉胶酶基因的全长DNA序列。PCR采用TaΚaRa公司的LA试剂盒,体系(总体积25μL)具体如下:10×LA Buffer II(Mg2+free),2.5μL;MgCl2(25mM),2.5μL;dNTP Mixture(各2.5mM),4μL;正向引物(10μM),1μL;反向引物(10μM),1μL;基因组模板(50ng/μL),1μL;LA-Taq(5U/μL),0.2μL;ddH2O,12.8μL。反应条件如下:预变性94℃5min;变性94℃30s;退火58℃30s;35个循环;延伸72℃3min(1Κb/min);延伸72℃10min;保温4℃。扩增结束后,1.2%琼脂糖凝胶电泳进行检测,上样量为3μL。随后对目的片段进行胶回收,连接到克隆载体pMD-18T上,连接产物转化大肠杆菌Top10感受态细胞,PCR进行阳性克隆筛选后测序,得到含有pMD-18T-原始编码序列的菌株。本发明得到海洋细菌C.lytica M9来源长度为2530bp的原始编码序列,其中包括一个完整的编码κ-卡拉胶酶基因的ORF(881-2368)。该基因DNA序列全长1488bp,编码495个氨基酸。该酶属于糖苷水解酶GH16家族。与已知κ-卡拉胶酶序列相似性最高为44%(NCBI:WP_013991622,Zobelliagalactanivorans),结果显示得到一种全新的海洋细菌来源κ-卡拉胶酶基因。
实施例2:海洋细菌C.lytica M9来源基因κ-卡拉胶酶基因的重组表达质粒和重组菌株的构建
将本发明获得的κ-卡拉胶酶基因克隆到原核表达载体pET-28a(+)中,构建重组表达质粒。首先基于获得的κ-卡拉胶酶基因的全长序列(采用软件预测ORF中的信号肽区域),设计获取目的基因成熟肽部分的上下游引物(上游引物Cly-κ-Car-F:CCCGAATTCCAAACATCTAATCCGAATGATAATT和下游引物Cly-κ-Car-R:GGCTCGAGCTATTGAATAAGCAGTTGTTTTG)。采用含有原始编码序列的质粒pMD-18T-原始编码序列模板,通过PCR方法获得目的基因成熟肽部分序列。采用限制性内切酶EcoR I和Xho I双酶切PCR产物,胶回收酶切之后的片段,跟同样经过EcoR I和Xho I双酶切的质粒pET-28a(+)链接,按照CaCl2转化法转化到大肠杆菌TOP10中,卡那霉素抗性筛选阳性克隆。采用质粒抽提试剂盒(宝生物)提取阳性克隆质粒,通过测序和EcoR I和Xho I双酶切鉴定,获得目的基因的重组表达质粒pET-28a(+)-Cly-κ-car。将该质粒进一步转化到大肠杆菌BL21中,构建重组表达工程菌株BL21-Cly-κ-CAR。
实施例3:利用重组表达菌株BL21-Cly-κ-CAR表达重组κ-卡拉胶酶
将活化好的1ml重组表达菌株BL21-Cly-κ-CAR转接到100ml含有20pg/ml卡那霉素的LB液体培养基中,37℃振荡培养(培养条件37℃,转速150r/min)至OD600达到0.6-0.8,将培养液温度降至18℃度左右,此时加入终浓度为0.l mM的IPTG进行诱导表达,诱导条件为18℃,转速100r/min,培养24h。离心收集菌体,将50ml菌体重悬于20ml海洋细菌C.lyticaM9发酵培养基中(每100ml陈海水中卡拉胶0.1%、蛋白胨0.5%、FeSO4.7H2O0.002%),在冰上进行超声波破碎处理,低温离心收集上清,上清液即为粗酶液,SDS-PAGE检测上清中目的基因的表达量。
实施例4:重组Cly-κ-CAR酶的活性检测
利用DNS(3,5一二硝基水杨酸)方法测定纯化的重组Cly-κ-CAR酶活性。具体操作:取1ml超声破碎后上清液即粗酶液,对照组酶液沸水浴5min灭活,对照组和实验组分别加入1ml浓度为0.2%(w/v)的κ-卡拉胶底物溶液,于45℃水浴反应30min,加入2ml DNS溶液,煮沸5min,迅速冷却后用紫外分光光度计于540nm下测定OD值,根据葡萄糖标准曲线求出反应液中的还原糖含量。测得的卡拉胶酶活性为70.07U/ml。另外,使用SDS-PAGE电泳对分别诱导了2h、4h、6h、8h的菌体进行检测,并用凝胶成像系统拍照,如图1所示,结果显示条带大小与理论预测的基本吻合。并配制含0.2%的κ-卡拉胶的SDS-PAGE电泳胶,进行正常的不连续SDS-PAGE电泳,电泳完毕,将凝胶取下先用预冷的蒸馏水漂洗,洗去电泳缓冲液,然后加入适量2.5%TritonX-100,摇床复性1h,倒掉之后,加入TritonX-100洗脱液洗脱30min,重复两次。倒掉洗脱液后加入适量孵育液,40℃孵育过夜后取出,预冷蒸馏水漂洗后,Alcianblue染色后蒸馏水脱色,直至出现清晰降解亮带,如图2所示,结果表明这个重组表达的Cly-κ-CAR酶是具有κ-卡拉胶降解活性的,为后续的研究和应用提供了良好材料。
<110> 大连大学
<120> 以海洋细菌为来源获取的κ-卡拉胶酶基因及重组酶制备方法
<160> 6
<170> PatentIn version 3.3
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<211> 1488
<212> DNA
<213> 人工合成
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atgtttcgaa acaacaatgt taattacaaa aaacagacta ctatgaaatt aaaaattatg 60
aaaccaaaaa aggtattttt aagttttctt ctggcattta tttgcttgct agggtacagc 120
caaaaaccaa acggacaaac atctaatccg aatgataatt ttaaattatt aaacgatttt 180
tcagatgaat ttaatacagg taacattaat tggagcaaat ggagtaaaac ggctaattta 240
ccaaacacaa aagcttggaa gtgggataac aatgccaatg ctaaaccggt aaattataaa 300
ggtgagcgtt ctgttgagct tactatgcgt caaaacgcca ataatgcaag agatggcatt 360
acatatttta aaagtggctg tttacaagct attaaacagt tgcctaaaaa ctttgtaggt 420
tatgtagaat ccagaattta tggtgcagaa attaactctc caaaagcaac aggtcttgac 480
aaatacagag gtgtgtgtcc gtctttttgg ttatacagta agttttttga taataaacca 540
attggtgagg ctgtatacac agaaattgat gttgtagaac tacaacaatt tgattttgat 600
cctaatggtc cggttgggca tcaacaagat ttaattacag atgcagaatc taatcttcat 660
ttagtaaaaa aagcaagttt tggtagagat tggtttagac caaaacaacc aaaagcaaga 720
gctgctcaat taaataagta tgagttacca ggtaaatttg atcctacaaa aggttggcat 780
acctatggtt gtgaaataac acctactaaa ttatattttt atgtagatgg cgttagagta 840
ggtagagctt tagataatac ttattggagt gataatccta tgtatgttat agcatcatta 900
ggattaagag taccatttgt agcgtttcaa ggtaatgtat ttgagcctgt gaacccagaa 960
gtaaatccta gagcaaaaaa gaatatagat gaaatgccag tatctatgca cgtagattat 1020
ataagagttt gggaaaaaaa tggagccgga aataacaatg ctaccaatgg caattgttca 1080
tctgtgcctg tttggaaaaa atctggagct ttttcaagag gagataaagt aaagcttaac 1140
aatgccattt atgaattaaa agctggtaca ggttcttgta gaccaggtgg agcttctggt 1200
tgttcttcaa accaatggac taaagtatct gactgtgcat ctaatagcag tattattaat 1260
accgacttag gaactgtata tccaaaccct gcgaatacag tagttaatgt ggtagctact 1320
aaaggagatt ttattagaat aattacttct gtgggtacag tagtacgtac tataaaagct 1380
aaaaatagta ctactataat agatatttca gcattaccgc caggtttgta tactgttaca 1440
attacaggta acaacaaaaa tgaaacaaaa caactgctta ttcaatag 1488
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MFRNNNVNYK KQTTMKLKIM KPKKVFLSFL LAFICLLGYS QKPNGQTSNP NDNFKLLNDF 60
SDEFNTGNIN WSKWSKTANL PNTKAWKWDN NANAKPVNYK GERSVELTMR QNANNARDGI 120
TYFKSGCLQA IKQLPKNFVG YVESRIYGAE INSPKATGLD KYRGVCPSFW LYSKFFDNKP 180
IGEAVYTEID VVELQQFDFD PNGPVGHQQD LITDAESNLH LVKKASFGRD WFRPKQPKAR 240
AAQLNKYELP GKFDPTKGWH TYGCEITPTK LYFYVDGVRV GRALDNTYWS DNPMYVIASL 300
GLRVPFVAFQ GNVFEPVNPE VNPRAKKNID EMPVSMHVDY IRVWEKNGAG NNNATNGNCS 360
SVPVWKKSGA FSRGDKVKLN NAIYELKAGT GSCRPGGASG CSSNQWTKVS DCASNSSIIN 420
TDLGTVYPNP ANTVVNVVAT KGDFIRIITS VGTVVRTIKA KNSTTIIDIS ALPPGLYTVT 480
ITGNNKNETK QLLIQ 495
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tcttgcttcg ctaccagctc 20
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tttggctctc ccaaaccaga 20
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cccgaattcc aaacatctaa tccgaatgat aatt 34
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<212> DNA
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ggctcgagct attgaataag cagttgtttt g 31
Claims (4)
1.一种以海洋细菌为来源获取的κ-卡拉胶酶基因,其特征在于,其核苷酸序列为SeqID.NO.1,该基因DNA序列全长1488bp,编码495个氨基酸,含有45个氨基酸的信号肽序列。
2.权利要求1所述的一种以海洋细菌为来源获取的κ-卡拉胶酶基因,其特征在于,从海洋细菌C.lytica M9中获取的方法包括如下步骤:
(1)根据海洋细菌C.lytica M9中16s RNA序列构建系统进化树,找到与目的菌株最相近且具有全基因组数据的参考菌株;
(2)根据基因组注释信息和NCBI中blast程序验证之后,找到参考菌株C.lytica DSM7489基因组中编码κ-卡拉胶酶的基因Celly_2915编号(gi|325284916:3333332-3334777蛋白序列ADY30732),同时确定该参考菌株中编码κ-卡拉胶酶的相邻上游基因Celly_2914编号(gi|325284916:3332347-3333021蛋白序列ADY30731)和下游基因Celly_2916编号(gi|325284916:3335359-3336312蛋白序列ADY30733)及分别对应的核苷酸和氨基酸序列;
(3)根据相邻上游基因Celly_2914和下游基因Celly_2916的氨基酸序列,通过BlocκMaκer在线软件程序进行比对和寻找保守核心区域,其中,Celly_2914的核心保守序列为:QGSINPM和Celly_2916的核心保守序列为:SGLGEPNE;
(4)根据Celly_2914基因的核心保守序列设计正向引物,
正向引物为:TCTTGCTTCGCTACCAGCTC;
根据根据Celly_2916基因的核心保守序列设计反向引物,
反向引物为:TTTGGCTCTCCCAAACCAGA;
(5)PCR扩增,以目的菌株C.lytica M9基因组为模板,利用步骤(4)中所述的正反向引物经一步PCR方法扩增,扩增产物切胶纯化,获得含有编码完整κ-卡拉胶酶基因的原始编码序列,具体操作为:
PCR体系具体如下:10×LA Buffer II Mg2+free,2.5μL;MgCl2 25mM,2.5μL;dNTPMixture各2.5mM,4μL;正向引物10μM,1μL;反向引物10μM,1μL;基因组模板50ng/μL,1μL;LA-Taq 5U/μL,0.2μL;ddH2O,12.8μL,总体积25μL;反应条件如下:预变性94℃ 5min;变性94℃ 30s;退火58℃ 30s;35个循环;延伸72℃ 3min、1Kb/min;延伸72℃ 10min;保温4℃;
扩增结束后,1.2%琼脂糖凝胶电泳进行检测,上样量为3μL,随后对目的片段进行胶回收,连接到克隆载体pMD-18T上,连接产物转化大肠杆菌Top10感受态细胞,PCR进行阳性克隆筛选后测序,得到含有pMD-18T-原始编码序列的菌株,得到海洋细菌C.lytica M9来源长度为2530bp的原始编码序列,其中包括一个完整的编码κ-卡拉胶酶基因的ORF(881-2368),该基因DNA序列全长1488bp,编码495个氨基酸,该酶属于糖苷水解酶GH16家族,与已知κ-卡拉胶酶序列相似性最高为44%,NCBI:WP_013991622,Zobellia galactanivorans,结果显示得到一种全新的海洋细菌来源κ-卡拉胶酶基因。
3.权利要求1所述的一种以海洋细菌为来源获取的κ-卡拉胶酶基因所编码的κ-卡拉胶酶,其特征在于,κ-卡拉胶酶的氨基酸序列为Seq ID.NO.2,属于糖苷水解酶GH16家族。
4.根据权利要求3所述的κ-卡拉胶酶,其特征在于,通过下述步骤制备而成:
1)、κ-卡拉胶酶基因的重组表达质粒和重组菌株的构建
(1)将κ-卡拉胶酶基因克隆到原核表达载体pET-28a(+)中,构建重组表达质粒,基于获得的κ-卡拉胶酶基因的全长序列,设计获取目的基因Cly-κ-car成熟肽部分的上下游引物:
上游引物Cly-κ-Car-F:CCCGAATTCCAAACATCTAATCCGAATGATAATT
下游引物Cly-κ-Car-R:GGCTCGAGCTATTGAATAAGCAGTTGTTTTG;
(2)采用含有原始编码序列的质粒pMD-18T-原始编码序列模板,通过PCR方法获得目的基因成熟肽部分序列;采用限制性内切酶EcoR I和Xho I双酶切PCR产物,胶回收酶切之后的片段,跟同样经过EcoR I和Xho I双酶切的质粒pET-28a(+)链接,按照CaCl2转化法转化到大肠杆菌TOP10中,卡那霉素抗性筛选阳性克隆;
(3)采用质粒抽提试剂盒提取阳性克隆质粒,通过测序和EcoR I和Xho I双酶切鉴定,获得目的基因的Cly-κ-car重组表达质粒pET-28a(+)-Cly-κ-car,将该质粒进一步转化到大肠杆菌BL21中,构建重组表达工程菌株BL21-Cly-κ-CAR;
2)、利用重组表达菌株BL21-Cly-κ-CAR表达重组κ-卡拉胶酶
将活化好的1ml重组表达菌株BL21-Cly-κ-CAR转接到100ml含有20pg/ml卡那霉素的LB液体培养基中,LB液体培养基为1000ml去离子水中加入胰蛋白胨10g、酵母提取物5g、NaCl10g,用5mol/LNaOH调pH至7.0,培养条件37℃,振荡培养,转速150r/min,至OD600达到0.6-0.8,将培养液温度降至18℃度左右,此时加入终浓度为0.l mM的IPTG进行诱导表达,诱导条件为18℃,转速100r/min,培养24h,离心收集菌体,将50ml菌体重悬于20ml海洋细菌C.lytica M9发酵培养基中,C.lytica M9发酵培养基为每100ml陈海水中加入卡拉胶0.1%、蛋白胨0.5%、FeSO4.7H2O 0.002%,在冰上进行超声波破碎处理,低温离心收集上清,上清液即为粗酶液,SDS-PAGE检测上清中目的基因的表达量;
(3)重组Cly-κ-CAR酶的活性检测。
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