CN113666991B - Yh66-rs07015基因改造得到的工程菌及其在制备缬氨酸中的应用 - Google Patents
Yh66-rs07015基因改造得到的工程菌及其在制备缬氨酸中的应用 Download PDFInfo
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- CN113666991B CN113666991B CN202110959115.3A CN202110959115A CN113666991B CN 113666991 B CN113666991 B CN 113666991B CN 202110959115 A CN202110959115 A CN 202110959115A CN 113666991 B CN113666991 B CN 113666991B
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Abstract
本发明公开了一种YH66‑RS07015基因改造得到的工程菌及其在制备缬氨酸中的应用。本发明提供了用于抑制YH66‑RS07015基因表达的物质或降低YH66‑RS07015蛋白丰度的物质或降低YH66‑RS07015蛋白活性的物质在提高细菌缬氨酸产量中的应用。本发明发现YH66‑RS07015蛋白对细菌的缬氨酸产量存在负调控,即YH66‑RS07015蛋白含量增高、缬氨酸产量降低,YH66‑RS07015蛋白含量降低、缬氨酸产量增高。抑制YH66‑RS07015基因表达可以提高缬氨酸产量,过表达YH66‑RS07015基因降低缬氨酸产量。进一步,本发明发现了YH66‑RS07015C1187T蛋白及其编码基因和应用。本发明对于缬氨酸工业化生产,具有重大的应用价值。
Description
技术领域
本发明属于生物技术领域,涉及一种YH66-RS07015基因改造得到的工程菌及其在制备缬氨酸中的应用,具体的所述改造为C1187T。
背景技术
缬氨酸是组成蛋白质的20种氨基酸之一,是人体必需的8种氨基酸和生糖氨基酸,它与其他两种高浓度氨基酸(异亮氨酸和亮氨酸)一起工作促进身体正常生长,修复组织,调节血糖,并提供需要的能量。在参加激烈体力活动时,缬氨酸可以给肌肉提供额外的能量产生葡萄糖,以防止肌肉衰弱。缬氨酸还帮助从肝脏清除多余的氮(潜在的毒素),并将身体需要的氮运输到各个部位。
缬氨酸是一种必需氨基酸,这意味着身体本身不能生产,必须通过膳食来源获得补充。它的天然食物来源包括谷物、奶制品、香菇、蘑菇、花生、大豆蛋白和肉类。尽管大多数人都可以从饮食中获得足够的数量,但是缬氨酸缺乏症的案例也屡见不鲜。当缬氨酸不足时,大脑中枢神经系统功能会发生紊乱,共济失调而出现四肢震颤。通过解剖切片脑组织,发现有红核细胞变性现象,晚期肝硬化病人因肝功能损害,易形成高胰岛素血症,致使血中支链氨基酸减少,支链氨基酸和芳香族氨基酸的比值由正常人的3.0-3.5降至1.0-1.5,故常用缬氨酸等支链氨基酸的注射液治疗肝功能衰竭以及酗酒和吸毒对这些器官造成的损害。此外,缬氨酸也可作为加快创伤愈合的治疗剂。L-缬氨酸,别名为2-氨基-3-甲基丁酸,CAS号为72-18-4,MDL号为MFCD00064220,EINECS号为200-773-6。目前制备L-缬氨酸主要是化学合成法。化学合成法的局限性:生产成本高,反应复杂,步骤多,且有许多副产物。
发明内容
本发明的目的是提供一种YH66-RS07015基因改造得到的工程菌及其在制备缬氨酸中的应用。
本发明提供了用于抑制YH66-RS07015基因表达的物质或降低YH66-RS07015蛋白丰度的物质或降低YH66-RS07015蛋白活性的物质的应用;
所述应用为如下(Ⅰ)或(Ⅱ)或(Ⅲ):
(Ⅰ)在提高细菌缬氨酸产量中的应用;
(Ⅱ)在生产缬氨酸中的应用;
(Ⅲ)在提高细菌菌量中的应用。
所述YH66-RS07015基因为编码YH66-RS07015蛋白的基因。
所述YH66-RS07015蛋白为如下(a1)或(a2)或(a3):
(a1)序列表的序列3所示的蛋白质;
(a2)来源于细菌且与(a1)具有95%以上同一性且与细菌产缬氨酸相关的蛋白质;
(a3)将(a1)所示的蛋白质经过一个或几个氨基酸残基的取代和/或缺失和/或添加得到的且与细菌产缬氨酸相关的由(a1)衍生的蛋白质。
这里使用的术语“同一性”指与天然氨基酸序列的序列相似性。同一性可以用肉眼或计算机软件进行评价。使用计算机软件,两个或多个序列之间的同一性可以用百分比(%)表示,其可以用来评价相关序列之间的同一性。
所述95%以上同一性具体可为96%以上同一性或97%以上同一性或98%以上同一性或99%以上同一性。
具体的,所述YH66-RS07015基因为如下(b1)或(b2)或(b3):
(b1)编码区如序列表的序列4所示的DNA分子;
(b2)来源于细菌且与(b1)具有95%以上同一性且编码所述蛋白质的DNA分子;
(b3)在严格条件下与(b1)杂交且编码所述蛋白质的DNA分子。
这里使用的术语“同一性”指与天然核酸序列的序列相似性。同一性可以用肉眼或计算机软件进行评价。使用计算机软件,两个或多个序列之间的同一性可以用百分比(%)表示,其可以用来评价相关序列之间的同一性。
所述95%以上同一性具体可为96%以上同一性或97%以上同一性或98%以上同一性或99%以上同一性。
所述严格条件可为在0.1×SSPE(或0.1×SSC),0.1%SDS的溶液中,在65℃条件下杂交并洗膜。
所述抑制YH66-RS07015基因表达可为敲除YH66-RS07015基因,也可为突变YH66-RS07015基因。
所述敲除可为敲除基因的部分区段,也可为敲除基因的整个编码框。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为序列表的序列5所示的DNA分子或具有序列表的序列5所示的DNA分子的重组质粒。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为序列表的序列8所示的DNA分子或具有序列表的序列8所示的DNA分子的重组质粒。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为实施例中的重组质粒pK18-YH66-RS07015C1187T或重组质粒pK18-ΔYH66-RS07015。
本发明还提供了一种重组菌,是抑制细菌中的YH66-RS07015基因表达得到的。
所述抑制细菌中的YH66-RS07015基因表达可为敲除细菌中的YH66-RS07015基因,也可为突变细菌中的YH66-RS07015基因。
所述敲除可为敲除基因的部分区段,也可为敲除基因的整个编码框。
示例性的,敲除细菌中的YH66-RS07015基因具体可为:使细菌基因组DNA中缺失序列表的序列4所示的DNA分子。
对于突变细菌中的YH66-RS07015基因,本领域普通技术人员可以很容易地采用已知的方法,例如定向突变或基因编辑等。
示例性的,突变细菌中的YH66-RS07015基因具体可为:使细菌基因组DNA中编码的YH66-RS07015蛋白的第396位氨基酸残基的密码子由编码T的密码子突变为编码其他氨基酸残基的密码子。具体的,所述其他氨基酸残基为I。
示例性的,突变细菌中的YH66-RS07015基因具体可为:使细菌基因组DNA中的YH66-RS07015基因发生如下点突变:第1187位核苷酸由C突变为其他核苷酸(具体可为T)。
示例性的,抑制细菌中的YH66-RS07015基因表达的实现方式可为:在细菌中导入用于抑制YH66-RS07015基因表达的物质。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为序列表的序列5所示的DNA分子或具有序列表的序列5所示的DNA分子的重组质粒。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为序列表的序列8所示的DNA分子或具有序列表的序列8所示的DNA分子的重组质粒。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为实施例中的重组质粒pK18-YH66-RS07015C1187T或重组质粒pK18-ΔYH66-RS07015。
本发明还保护所述重组菌在制备缬氨酸中的应用。
本发明还保护一种制备缬氨酸的方法,包括如下步骤:发酵所述重组菌。
本领域技术人员可以采用现有技术中的发酵方法进行发酵。也可通过常规试验进行发酵方法的优化和改进。可以在本领域中已知的发酵条件下在合适的培养基中进行细菌的发酵。培养基可以包含:碳源、氮源、微量元素、及其组合。在培养中,可以调节培养物的pH。此外,培养时可以包括防止气泡产生,例如通过使用消泡剂进行气泡产生的防止。此外,培养时可以包括将气体注射入培养物中。气体可以包括能够维持培养物的需氧条件的任何气体。在培养中,培养物的温度可以是20至45℃。
所述方法还可包括如下步骤:从培养物中获得缬氨酸。从培养物中获得缬氨酸可通过各种方式实现,包括但不限于:用硫酸或氢氯酸等处理培养物,接着进行诸如阴离子交换层析、浓缩、结晶和等电点沉淀的方法的组合。
所述发酵中,示例性的发酵培养基的配方见表3,余量为水。
所述发酵中,示例性的发酵控制工艺见表4。
示例性的,所述发酵中,完成接种的初始时刻,体系OD值可为0.3-0.5。
示例性的,所述发酵的发酵过程中:用于调pH的为氨水;发酵体系中有泡沫时,加入适量消泡剂antifoam(CB-442);通过补加70%葡萄糖水溶液控制体系含糖量(残糖)。
本发明还提供了一种提高细菌的缬氨酸产量的方法,包括如下步骤:抑制细菌中的YH66-RS07015基因表达或降低细菌中YH66-RS07015蛋白丰度或降低细菌中YH66-RS07015蛋白活性。
所述抑制细菌中的YH66-RS07015基因表达可为敲除细菌中的YH66-RS07015基因,也可为突变细菌中的YH66-RS07015基因。
所述敲除可为敲除基因的部分区段,也可为敲除基因的整个编码框。
示例性的,敲除细菌中的YH66-RS07015基因具体可为:使细菌基因组DNA中缺失序列表的序列4所示的DNA分子。
对于突变细菌中的YH66-RS07015基因,本领域普通技术人员可以很容易地采用已知的方法,例如定向突变或基因编辑等。
示例性的,突变细菌中的YH66-RS07015基因具体可为:使细菌基因组DNA中编码的YH66-RS07015蛋白的第396位氨基酸残基的密码子由编码T的密码子突变为编码其他氨基酸残基的密码子。具体的,所述其他氨基酸残基为I。
示例性的,突变细菌中的YH66-RS07015基因具体可为:使细菌基因组DNA中的YH66-RS07015基因发生如下点突变:第1187位核苷酸由C突变为其他核苷酸(具体可为T)。
示例性的,抑制细菌中的YH66-RS07015基因表达的实现方式可为:在细菌中导入用于抑制YH66-RS07015基因表达的物质。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为序列表的序列5所示的DNA分子或具有序列表的序列5所示的DNA分子的重组质粒。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为序列表的序列8所示的DNA分子或具有序列表的序列8所示的DNA分子的重组质粒。
示例性的,所述用于抑制YH66-RS07015基因表达的物质具体可为实施例中的重组质粒pK18-YH66-RS07015C1187T或重组质粒pK18-ΔYH66-RS07015。
本发明还保护YH66-RS07015蛋白在调控细菌的缬氨酸产量中的应用。
所述调控为负调控,即YH66-RS07015蛋白含量增高,缬氨酸产量降低。
所述调控为负调控,即YH66-RS07015蛋白含量降低,缬氨酸产量增高。
本发明还保护YH66-RS07015蛋白在调控细菌的菌量中的应用。
所述调控为负调控,即YH66-RS07015蛋白含量增高,细菌菌量降低。
所述调控为负调控,即YH66-RS07015蛋白含量降低,细菌菌量增高。
本发明还保护一种突变蛋白,命名为YH66-RS07015C1187T蛋白,是将YH66-RS07015蛋白第396位氨基酸残基由T突变为其他氨基酸残基得到的。
具体的,所述其他氨基酸残基为I。
示例性的,所述YH66-RS07015C1187T蛋白如序列表的序列1所示。
本发明还保护YH66-RS07015C1187T蛋白的编码基因或具有所述YH66-RS07015C1187T蛋白的编码基因的表达盒或具有所述YH66-RS07015C1187T蛋白的编码基因的重组载体或具有所述YH66-RS07015C1187T蛋白的编码基因的重组菌。
YH66-RS07015C1187T蛋白的编码基因,命名为YH66-RS07015C1187T基因。
具体的,所述YH66-RS07015C1187T基因为如下(c1)或(c2)或(c3):
(c1)编码区如序列表的序列2所示的DNA分子;
(c2)来源于细菌且与(c1)具有95%以上同一性且编码所述蛋白质的DNA分子;
(c3)在严格条件下与(c1)杂交且编码所述蛋白质的DNA分子。
这里使用的术语“同一性”指与天然核酸序列的序列相似性。同一性可以用肉眼或计算机软件进行评价。使用计算机软件,两个或多个序列之间的同一性可以用百分比(%)表示,其可以用来评价相关序列之间的同一性。
所述95%以上同一性具体可为96%以上同一性或97%以上同一性或98%以上同一性或99%以上同一性。
所述严格条件可为在0.1×SSPE(或0.1×SSC),0.1%SDS的溶液中,在65℃条件下杂交并洗膜。
本发明还保护YH66-RS07015C1187T蛋白、YH66-RS07015C1187T基因、具有YH66-RS07015C1187T基因的表达盒或具有YH66-RS07015C1187T基因的重组载体或具有YH66-RS07015C1187T基因的重组菌在制备缬氨酸中的应用。
本发明还保护一种提高细菌的缬氨酸产量的方法,包括如下步骤:使细菌基因组DNA中编码的YH66-RS07015蛋白的第396位氨基酸残基的密码子由编码T的密码子突变为编码其他氨基酸残基的密码子。
具体的,所述其他氨基酸残基为I。
所述方法具体包括如下步骤:使细菌基因组DNA中的YH66-RS07015基因发生如下点突变:第1187位核苷酸由C突变为其他核苷酸(具体可为T)。
所述方法具体包括如下步骤:在细菌中导入序列表的序列5所示的DNA分子或具有序列表的序列5所示的DNA分子的重组质粒。
以上任一所述细菌包括但不限于如下:棒杆菌属细菌,优选嗜乙酰棒杆菌(Corynebacteriumacetoacidophilum)、醋谷棒杆菌(Corynebacteriumacetoglutamicum)、美棒杆菌(Corynebacteriumcallunae)、谷氨酸棒杆菌(Corynebacteriumglutamicum)、黄色短杆菌(Brevibacteriumflavum)、乳糖发酵短杆菌(Brevibacteriumlactofermentum)、产氨棒杆菌(Corynebacterium ammoniagenes)、北京棒杆菌(Corynebacteriumpekinense)、解糖短杆菌(Brevibacteriumsaccharolyticum)、玫瑰色短杆菌(Brevibacteriumroseum)、生硫短杆菌(Brevibacteriumthiogenitalis)。
以上任一所述细菌为具有生产缬氨酸的能力的细菌。
“具有生产缬氨酸的能力的细菌”是指细菌具有以下能力:在培养基和/或细菌的细胞中产生并累积缬氨酸的能力。从而,当细菌在培养基中培养时可以收集缬氨酸。
所述细菌可为自然采集的野生型细菌也可为修饰后的细菌。
“修饰后的细菌”指的是将自然采集的野生型细菌进行人工突变和/或诱变得到的改造后的细菌。
具体的,所述谷氨酸棒杆菌可为谷氨酸棒杆菌CGMCC21260。
谷氨酸棒杆菌(Corynebacteriumglutamicum)YPFV1,已于2020年11月30日保藏于中国微生物菌种保藏管理委员会普通微生物中心(简称CGMCC,地址为:北京市朝阳区北辰西路1号院3号,中国科学院微生物研究所),保藏登记号为CGMCC No.21260。谷氨酸棒杆菌(Corynebacteriumglutamicum)YPFV1,又称为谷氨酸棒杆菌CGMCC21260。
以上任一所述缬氨酸的含义为广义的缬氨酸,包括游离形式缬氨酸、缬氨酸的盐或两者的混合物。
具体的,所述缬氨酸为L-缬氨酸。
以上任何方法或应用还可用于缬氨酸的下游产品的制备。
谷氨酸棒杆菌中的YH66-RS07015蛋白如序列表的序列3所示,其编码基因如序列表的序列4所示。本发明中通过引入点突变,得到了序列表的序列1所示的YH66-RS07015C1187T蛋白,YH66-RS07015C1187T蛋白的编码基因如序列表的序列2所示。与YH66-RS07015基因相比,YH66-RS07015C1187T基因的差异在于第1187位核苷酸由C突变为T。与YH66-RS07015蛋白相比,YH66-RS07015C1187T蛋白的差异在于第396位氨基酸残基由T突变为突变为I。
本发明发现YH66-RS07015蛋白对细菌的缬氨酸产量存在负调控,即YH66-RS07015蛋白含量增高、缬氨酸产量降低,YH66-RS07015蛋白含量降低、缬氨酸产量增高。抑制YH66-RS07015基因表达可以提高缬氨酸产量,过表达YH66-RS07015基因降低缬氨酸产量。进一步,本发明发现了YH66-RS07015C1187T蛋白及其编码基因和应用。本发明对于缬氨酸工业化生产,具有重大的应用价值。
具体实施方式
下面结合具体实施方式对本发明进行进一步的详细描述,给出的实施例仅为了阐明本发明,而不是为了限制本发明的范围。以下提供的实施例可作为本技术领域普通技术人员进行进一步改进的指南,并不以任何方式构成对本发明的限制。
下述实施例中的实验方法,如无特殊说明,均为常规方法,按照本领域内的文献所描述的技术或条件或者按照产品说明书进行。下述实施例中所用的材料、试剂等,如无特殊说明,均可从商业途径得到。pK18mobsacB质粒:Addgene公司;pK18mobsacB质粒中具有卡那霉素抗性基因作为筛选标记。pXMJ19质粒:BioVector质粒载体菌种细胞基因保藏中心;pXMJ19质粒中具有氯霉素抗性基因作为筛选标记。NEBuilder酶:NEB公司。如无特殊说明,实施例中的培养基为配方为表1的培养基(余量为水,pH为7.0)。不含卡那霉素培养基即表1所示的培养基。含卡那霉素的培养基由表1所示的培养基和卡那霉素组成,卡那霉素的含量为50μg/ml。如无特殊说明,实施例中的培养指的是32℃静置培养。实施例中的单链构象多态性聚丙烯酰胺凝胶电泳(sscp-PAGE):采用的胶浓度为8%,电泳胶的组成见表2;电泳条件为:使用1×TBE缓冲液,120V电压,电泳时间10h。
如无特殊说明,以下实施例中的定量试验,均设置三次重复实验,结果取平均值。
表1
| 组分 | 在培养基中的浓度 |
| 蔗糖 | 10g/L |
| 多聚蛋白胨 | 10g/L |
| 牛肉膏 | 10g/L |
| 酵母粉 | 5g/L |
| 尿素 | 2g/L |
| 氯化钠 | 2.5g/L |
| 琼脂粉 | 20g/L |
表2
| 组分 | 加入量 |
| 40%丙烯酰胺 | 8mL |
| ddH2O | 26mL |
| 甘油 | 4mL |
| 10×TBE | 2mL |
| TEMED | 40μL |
| 10%AP | 600μL |
实施例1、谷氨酸棒杆菌CGMCC21260的获得
谷氨酸棒杆菌ATCC15168:ATCC中编号为15168的谷氨酸棒杆菌(Corynebacteriumglutamicum)。
将谷氨酸棒杆菌ATCC15168进行诱变,获得谷氨酸棒杆菌(Corynebacteriumglutamicum)YPFV1。
谷氨酸棒杆菌(Corynebacterium glutamicum)YPFV1,已于2020年11月30日保藏于中国微生物菌种保藏管理委员会普通微生物中心(简称CGMCC,地址为:北京市朝阳区北辰西路1号院3号,中国科学院微生物研究所),保藏登记号为CGMCC No.21260。谷氨酸棒杆菌(Corynebacterium glutamicum)YPFV1,又称为谷氨酸棒杆菌CGMCC21260。
实施例2、构建重组菌YPV-007
P1:5'-CAGTGCCAAGCTTGCATGCCTGCAGGTCGACTCTAGGCCAAGATCGGCACCGGTGG-3';
P2:5'-CCTCTTGCTTGATCCAGATGGAGGAAGGCACGAC-3';
P3:5'-GTCGTGCCTTCCTCCATCTGGATCAAGCAAGAGG-3';
P4:5'-CAGCTATGACCATGATTACGAATTCGAGCTCGGTACCCGTGAGGAGAAGACAGCGCGG-3'。
P5:5'-CGACATCAAGATCGACACCG-3';
P6:5'-GCAGAGCGCTCGCCTGGCTT-3'。
一、构建重组质粒
1、以谷氨酸棒杆菌ATCC15168为模板,采用引物P1和引物P2组成的引物对进行PCR扩增,回收扩增产物(628bp)。
2、以谷氨酸棒杆菌ATCC15168为模板,采用引物P3和引物P4组成的引物对进行PCR扩增,回收扩增产物(620bp)。
3、同时将步骤1回收的扩增产物和步骤2回收的扩增产物作为模板,采用引物P1和引物P4组成的引物对进行PCR扩增(Overlap PCR),回收扩增产物(1214bp)。经测序,扩增产物如序列表的序列5所示。
4、取pK18mobsacB质粒,采用限制性内切酶Xba I进行单酶切,回收线性化质粒。
5、将步骤3回收的扩增产物与步骤4回收的线性化质粒共孵育(采用NEBuilder酶,50℃孵育30min),得到重组质粒pK18-YH66-RS07015C1187T。经测序验证,重组质粒pK18-YH66-RS07015C1187T中具有序列表的序列5所示的DNA分子。
二、构建重组菌YPV-007
1、采用重组质粒pK18-YH66-RS07015C1187T对谷氨酸棒杆菌CGMCC21260进行电击转化,然后培养。
2、挑取步骤1中的菌株,采用含15%蔗糖的培养基培养,然后挑取单菌落,分别采用含卡那霉素的培养基和不含卡那霉素的培养基进行培养,筛选在含卡那霉素的培养基上不能生长且在不含卡那霉素的培养基上可以生长的菌株。
3、取步骤2筛选的菌株,采用引物P5和引物P6组成的引物对进行PCR扩增,然后回收扩增产物(270bp)。
4、取步骤3的扩增产物,先95℃变性10min再冰浴5min,然后进行sscp-PAGE。电泳时,采用重组质粒pK18-YH66-RS07015C1187T的扩增片段(即以重组质粒pK18-YH66-RS07015C1187T为模板,采用引物P5和引物P6组成的引物对进行PCR扩增的扩增产物)为阳性对照,采用谷氨酸棒杆菌CGMCC21260的扩增片段(即以谷氨酸棒杆菌CGMCC21260为模板,采用引物P5和引物P6组成的引物对进行PCR扩增的扩增产物)为阴性对照,水作为空白对照。由于片段结构不同,电泳位置不同,电泳位置与阴性对照不一致且与阳性对照一致的菌株为筛选的目的菌株(等位替换成功的重组菌株)。
5、根据步骤4的结果,将筛选得到的菌株的步骤3的扩增产物进行测序验证,得到重组菌YPV-007。与谷氨酸棒杆菌CGMCC21260相比,重组菌YPV-007的差异仅在于将谷氨酸棒杆菌CGMCC21260基因组中的序列表的序列4所示的YH66-RS07015基因取代为了序列表的序列2所示的YH66-RS07015C1187T突变基因。序列2和序列4仅存在一个核苷酸差异,位于第1187位。重组菌YPV-007即将谷氨酸棒杆菌CGMCC21260中的YH66-RS07015基因进行突变(单点突变)得到的工程菌株。
实施例2、构建重组菌YPV-009和重组菌YPV-008
P7:5'-CAGTGCCAAGCTTGCATGCCTGCAGGTCGACTCTAGCATGACGGCTGACTGGACTC-3';
P8:5'-TGAAATGTAAGATTCAAAGAAATCGGACTCCTTAAATGGG-3';
P9:5'-CCCATTTAAGGAGTCCGATTTCTTTGAATCTTACATTTCA-3';
P10:5'-CTATGTGAGTAGTCGATTTATTAGATATCTGCAGGTGAGG-3';
P11:5'-CCTCACCTGCAGATATCTAATAAATCGACTACTCACATAG-3';
P12:5'-CAGCTATGACCATGATTACGAATTCGAGCTCGGTACCCTGCATAAGAAACAACCACTT-3'。
P13:5'-GTCCGCTCTGTTGGTGTTCA-3';
P14:5'-GATTGCTTCGCCGCGGTATT-3'。
P15:5'-TCCCACACCTCTACTCACGG-3';
P16:5'-TGGAGGAATATTCGGCCCAG-3'。
一、构建重组菌YPV-009
1、以重组菌YPV-007为模板,采用引物P7和引物P8组成的引物对进行PCR扩增,回收扩增产物(806bp)。
2、以重组菌YPV-007为模板,采用引物P9和引物P10组成的引物对进行PCR扩增,回收扩增产物(1739bp)。
3、以重组菌YPV-007为模板,采用引物P11和引物P12组成的引物对进行PCR扩增,回收扩增产物(783bp)。
4、取pK18mobsacB质粒,采用限制性内切酶Xba I进行单酶切,回收线性化质粒。
5、将步骤1回收的扩增产物、步骤2回收的扩增产物、步骤3回收的扩增产物与步骤4回收的线性化质粒共孵育(采用NEBuilder酶,50℃孵育30min),得到重组质粒009。经测序验证,重组质粒009中具有序列表的序列6所示的DNA分子。
6、采用重组质粒009对谷氨酸棒杆菌CGMCC21260进行电击转化,然后培养,然后对各个单菌落分别进行PCR鉴定(采用引物P13和引物P14组成的引物对),能扩增出1755bp条带的菌株为阳性菌株。
7、挑取步骤6中的阳性菌株,采用含15%蔗糖的培养基培养,然后挑取单菌落,分别采用含卡那霉素的培养基和不含卡那霉素的培养基进行培养,筛选在含卡那霉素的培养基上不能生长且在不含卡那霉素的培养基上可以生长的菌株。
8、取步骤7筛选的菌株,采用引物P15和引物P16组成的引物对进行PCR扩增,扩增出1804bp条带的菌株为YH66-RS07015C1187T基因整合到谷氨酸棒杆菌CGMCC21260基因组上的阳性菌株,将其命名为重组菌YPV-009。重组菌YPV-009为基因组上过表达YH66-RS07015C1187T基因的工程菌株。
二、构建重组菌YPV-008
将模板均由“重组菌YPV-007”替换为“谷氨酸棒杆菌ATCC15168”,其他同步骤一。
得到YH66-RS07015基因整合到谷氨酸棒杆菌CGMCC21260基因组上的阳性菌株,将其命名为重组菌YPV-008。重组菌YPV-008为基因组上过表达YH66-RS07015基因的工程菌株。与重组菌YPV-009相比,重组菌YPV-008的差异仅在于:整合到谷氨酸棒杆菌CGMCC21260基因组的外源DNA的序列中,序列4取代了序列2。
实施例3、构建重组菌YPV-011和重组菌YPV-010
一、构建重组菌YPV-011
1、以重组菌YPV-007为模板,采用引物P17和引物P18组成的引物对进行PCR扩增,回收扩增产物(1769bp)。经测序,扩增产物如序列表的序列7所示。
P17:5'-GCTTGCATGCCTGCAGGTCGACTCTAGAGGATCCCCTCTTTGAATCTTACATTTCA-3';
P18:5'-ATCAGGCTGAAAATCTTCTCTCATCCGCCAAAACTTAGATATCTGCAGGTGAGG-3'。
2、取pXMJ19质粒,采用限制性内切酶EcoR I酶切进行单酶切,回收线性化质粒。
3、将步骤1回收的扩增产物与步骤2回收的线性化质粒共孵育(采用NEBuilder酶,50℃孵育30min),得到重组质粒pXMJ19-YH66-RS07015C1187T。经测序验证,重组质粒pXMJ19-YH66-RS07015C1187T中具有序列表的序列7所示的DNA分子。
4、将重组质粒pXMJ19-YH66-RS07015C1187T电转导入谷氨酸棒杆菌CGMCC21260,得到重组菌YPV-011。重组菌YPV-011为通过质粒过表达YH66-RS07015C1187T基因的工程菌株。
二、构建重组菌YPV-010
将模板由“重组菌YPV-007”替换为“谷氨酸棒杆菌ATCC15168”,其他同步骤一。
得到重组菌YPV-010。重组菌YPV-010为通过质粒过表达YH66-RS07015基因的工程菌株。与重组菌YPV-011相比,重组菌YPV-010的差异仅在于:通过质粒过表达的外源DNA的序列中,序列4取代了序列2。
实施例4、构建基因组上缺失YH66-RS07015基因的工程菌株
P19:5'-CAGTGCCAAGCTTGCATGCCTGCAGGTCGACTCTAGTAGGCGGCAAAAACGCGCGC-3';
P20:5'-CATTCTTTTTCTAGCCTTCCGGAACTCACCGTCCTTACAG-3';
P21:5'-CTGTAAGGACGGTGAGTTCCGGAAGGCTAGAAAAAGAATG-3';
P22:5'-CAGCTATGACCATGATTACGAATTCGAGCTCGGTACCCAAATGCACCCCGCGACAATG-3'。
P23:5'-TAGGCGGCAAAAACGCGCGC-3';
P24:5'-AAATGCACCCCGCGACAATG-3'。
一、构建重组质粒
1、以谷氨酸棒杆菌ATCC15168为模板,采用引物P19和引物P20组成的引物对进行PCR扩增,回收扩增产物(上游同源臂片段,764bp)。
2、以谷氨酸棒杆菌ATCC15168为模板,采用引物P21和引物P22组成的引物对进行PCR扩增,回收扩增产物(下游同源臂片段,724bp)。
3、同时将步骤1回收的扩增产物和步骤2回收的扩增产物作为模板,采用引物P19和引物P22组成的引物对进行PCR扩增(Overlap PCR),回收扩增产物(1448bp)。经测序,扩增产物如序列表的序列8所示。
4、取pK18mobsacB质粒,采用限制性内切酶Xba I进行单酶切,回收线性化质粒。
5、将步骤3回收的扩增产物与步骤4回收的线性化质粒共孵育(采用NEBuilder酶,50℃孵育30min),得到重组质粒pK18-ΔYH66-RS07015。经测序,重组质粒pK18-ΔYH66-RS07015中具有序列表的序列8所示的DNA分子。
二、构建重组菌YPV-012
1、采用重组质粒pK18-ΔYH66-RS07015对谷氨酸棒杆菌CGMCC21260进行电击转化,然后培养,然后对各个单菌落分别进行PCR鉴定(采用引物P23和引物P24组成的引物对)。能同时扩增出1374bp及2820bp条带的菌株为阳性菌株。只扩增出2820bp条带的菌株为转化失败的出发菌,其中的2820bp片段如序列表的序列9所示。
2、挑取步骤1中的阳性菌株,采用含15%蔗糖的培养基培养,然后挑取单菌落,分别采用含卡那霉素的培养基和不含卡那霉素的培养基进行培养,筛选在含卡那霉素的培养基上不能生长且在不含卡那霉素的培养基上可以生长的菌株。
3、取步骤2筛选的菌株,采用引物P23和引物P24组成的引物对进行PCR扩增,仅显示一种扩增产物且大小为1374bp的菌株为YH66-RS07015基因编码区被敲除的阳性菌株。
4、将步骤3筛选得到的菌株,再次采用引物P23和引物P24组成的引物对进行PCR扩增并测序,将测序正确的菌株命名为重组菌YPV-012。与谷氨酸棒杆菌CGMCC21260的基因组DNA相比,重组菌YPV-012的差异仅在于缺失了序列表的序列4所示的DNA分子。
实施例5、发酵制备L-缬氨酸
供试菌株分别为:谷氨酸棒杆菌CGMCC21260、重组菌YPV-007、重组菌YPV-008、重组菌YPV-009、重组菌YPV-010、重组菌YPV-011和重组菌YPV-012。
发酵罐:BLBIO-5GC-4-H型号的发酵罐(上海百仑生物科技有限公司)。
发酵培养基的配方见表3,余量为水。
表3发酵培养基配方
| 成分 | 含量 |
| 硫酸铵 | 14g/L |
| 磷酸二氢钾 | 1g/L |
| 磷酸氢二钾 | 1g/L |
| 硫酸镁 | 0.5g/L |
| 酵母粉 | 2g/L |
| 硫酸亚铁 | 18mg/L |
| 硫酸锰 | 4.2mg/L |
| 生物素 | 0.02mg/L |
| 维生素B1 | 2mg/L |
| 消泡剂antifoam(CB-442) | 0.5mL/L |
| 葡萄糖(底糖) | 40g/L |
发酵控制工艺见表4。
完成接种的初始时刻,体系OD值为0.3-0.5。
发酵过程中:用于调pH的为氨水;发酵体系中有泡沫时,加入适量消泡剂antifoam(CB-442);通过补加70%葡萄糖水溶液控制体系含糖量(残糖)。
表4发酵控制工艺
完成发酵后,收集上清,采用HPLC检测上清中的L-缬氨酸产量。
结果见表5。重组菌YPV-007和重组菌YPV-012的L-缬氨酸产量显著高于谷氨酸棒杆菌CGMCC21260。结果表明,抑制YH66-RS07015基因表达可以提高L-缬氨酸产量,过表达YH66-RS07015基因降低L-缬氨酸产量。
表5 L-缬氨酸发酵实验结果
| 菌株 | OD610 | L-缬氨酸产量(g/L) |
| 谷氨酸棒杆菌CGMCC21260 | 98.2 | 82.1 |
| 重组菌YPV-007 | 98.9 | 85.8 |
| 重组菌YPV-008 | 97.6 | 80.7 |
| 重组菌YPV-009 | 97.8 | 80.4 |
| 重组菌YPV-010 | 97.2 | 79.5 |
| 重组菌YPV-011 | 97.4 | 80.5 |
| 重组菌YPV-012 | 99.5 | 85.2 |
以上对本发明进行了详述。对于本领域技术人员来说,在不脱离本发明的宗旨和范围,以及无需进行不必要的实验情况下,可在等同参数、浓度和条件下,在较宽范围内实施本发明。虽然本发明给出了特殊的实施例,应该理解为,可以对本发明作进一步的改进。总之,按本发明的原理,本申请欲包括任何变更、用途或对本发明的改进,包括脱离了本申请中已公开范围,而用本领域已知的常规技术进行的改变。按以下附带的权利要求的范围,可以进行一些基本特征的应用。
序列表
<110> 宁夏伊品生物科技股份有限公司
<120> YH66-RS07015基因改造得到的工程菌及其在制备缬氨酸中的应用
<130> GNCYX211993
<160> 9
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Lys Ala Leu Gln Tyr Met Asp Leu Val Pro Gly Thr Pro Leu Arg Asp
340 345 350
Ile Lys Ile Asp Thr Val Phe Leu Gly Ser Cys Thr Asn Ala Arg Ile
355 360 365
Glu Asp Leu Gln Ile Ala Ala Asp Ile Leu Lys Gly His Lys Ile Ala
370 375 380
Asp Gly Met Arg Met Met Val Val Pro Ser Ser Thr Trp Ile Lys Gln
385 390 395 400
Glu Ala Glu Ala Leu Gly Leu Asp Lys Ile Phe Thr Asp Ala Gly Ala
405 410 415
Glu Trp Arg Thr Ala Gly Cys Ser Met Cys Leu Gly Met Asn Pro Asp
420 425 430
Gln Leu Lys Pro Gly Glu Arg Ser Ala Ser Thr Ser Asn Arg Asn Phe
435 440 445
Glu Gly Arg Gln Gly Pro Gly Gly Arg Thr His Leu Val Ser Pro Ala
450 455 460
Val Ala Ala Ala Thr Ala Ile Arg Gly Thr Leu Ser Ser Pro Ala Asp
465 470 475 480
Ile
<210> 4
<211> 1446
<212> DNA
<213> Corynebacterium glutamicum
<400> 4
atgaccagcc ccgtggagaa cagcacctca actgagaagc tgaccctggc agagaaggtg 60
tggcgcgacc atgtcgtgtc caagggagaa aacggcgagc ccgacctcct ctacatcgac 120
ctgcagctgc tgcatgaagt gacctcacca caggcattcg acggcctgcg catgactggc 180
cgcaaactgc gccacccaga actgcacctg gccaccgaag accacaacgt gccaaccgaa 240
ggcatcaaga ctggctcact gctggaaatc aacgaccaga tttcccgcct gcaggtatcc 300
accctgcgcg acaactgtga agagttcggt gttcgcctgc acccaatggg tgatgtccgc 360
cagggcatcg tgcacaccgt tggcccacag ctgggcgcaa ctcagccggg catgaccatt 420
gtgtgcggtg actcccacac ctctactcac ggcgcgtttg gctccatggc attcggtatc 480
ggtacctctg aggttgagca cgtcatggcc actcagaccc tgccattgaa gcctttcaag 540
accatggcca ttgaagttac tggcgaactg cagccaggtg tttcctccaa ggacctgatc 600
ctggcgatca ttgccaagat cggcaccggt ggtggacaag gctacgttct ggaataccgc 660
ggcgaagcaa tccgcaagat gtccatggat gcacgcatga ccatgtgcaa catgtccatc 720
gaagctggcg cacgtgccgg catgatcgcc ccagaccaaa ccaccttcga ctacgttgaa 780
ggccgcgaaa tggcaccaaa gggcgccgac tgggacgaag cagttgctta ctggaagacc 840
ctgccaaccg acgaaggcgc aacctttgac aaggtcgtag aaatcgatgg ctccgcactg 900
accccattca tcacctgggg caccaaccca ggccaaggtc tgccactgag cgaaaccgtg 960
ccaaacccag aagacttcac caacgacaac gacaaggcag cagccgaaaa ggcactgcag 1020
tacatggacc tggtaccagg aaccccactg cgcgacatca agatcgacac cgtcttcctg 1080
ggatcctgca ccaacgcccg catcgaagac ctgcagatcg ccgctgacat cctcaagggc 1140
cacaaaatcg ccgacggcat gcgcatgatg gtcgtgcctt cctccacctg gatcaagcaa 1200
gaggccgaag cactcggact ggacaaaatc ttcaccgacg ctggcgctga atggcgtacc 1260
gcaggctgct ccatgtgcct gggcatgaac ccagaccaac tgaagccagg cgagcgctct 1320
gcatccacct ccaaccgaaa cttcgaagga cgccaaggac caggaggccg cacccacctg 1380
gtatccccag cagtcgcagc cgccaccgca atccgcggca ccctgtcctc acctgcagat 1440
atctaa 1446
<210> 5
<211> 1214
<212> DNA
<213> 人工序列(Artificial Sequence)
<400> 5
cagtgccaag cttgcatgcc tgcaggtcga ctctaggcca agatcggcac cggtggtgga 60
caaggctacg ttctggaata ccgcggcgaa gcaatccgca agatgtccat ggatgcacgc 120
atgaccatgt gcaacatgtc catcgaagct ggcgcacgtg ccggcatgat cgccccagac 180
caaaccacct tcgactacgt tgaaggccgc gaaatggcac caaagggcgc cgactgggac 240
gaagcagttg cttactggaa gaccctgcca accgacgaag gcgcaacctt tgacaaggtc 300
gtagaaatcg atggctccgc actgacccca ttcatcacct ggggcaccaa cccaggccaa 360
ggtctgccac tgagcgaaac cgtgccaaac ccagaagact tcaccaacga caacgacaag 420
gcagcagccg aaaaggcact gcagtacatg gacctggtac caggaacccc actgcgcgac 480
atcaagatcg acaccgtctt cctgggatcc tgcaccaacg cccgcatcga agacctgcag 540
atcgccgctg acatcctcaa gggccacaaa atcgccgacg gcatgcgcat gatggtcgtg 600
ccttcctcca tctggatcaa gcaagaggcc gaagcactcg gactggacaa aatcttcacc 660
gacgctggcg ctgaatggcg taccgcaggc tgctccatgt gcctgggcat gaacccagac 720
caactgaagc caggcgagcg ctctgcatcc acctccaacc gaaacttcga aggacgccaa 780
ggaccaggag gccgcaccca cctggtatcc ccagcagtcg cagccgccac cgcaatccgc 840
ggcaccctgt cctcacctgc agatatctaa ggaaggctag aaaaagaatg gaaaaattta 900
ccacccacac cggcgttggc gttccactgc agcgatccaa cgtggacacc gaccagatca 960
tccccgccgt ctacctcaag cgcgtcaccc gcacaggctt cgaagacgga ctgttttcca 1020
actggcgcca aaacgacccc aactttgtcc tcaacaccga cacctacaag aacggctccg 1080
ttctcgtagc aggccctgac tttggcaccg gctcctcccg cgagcacgcc gtctgggcac 1140
tcatggacta cggcttccgc gctgtcttct cctcacgggt accgagctcg aattcgtaat 1200
catggtcata gctg 1214
<210> 6
<211> 3248
<212> DNA
<213> 人工序列(Artificial Sequence)
<400> 6
cagtgccaag cttgcatgcc tgcaggtcga ctctagcatg acggctgact ggactcgact 60
tccatacgag gttctggaga agatctccac ccgcatcacc aacgaagttc cagatgtgaa 120
ccgcgtggtt ttggacgtaa cctccaagcc accaggaacc atcgaatggg agtaggcctt 180
aaatgagcct tcgttaagcg gcaatcacct tattggagat tgtcgctttt cccatttctc 240
cgggttttct ggaacttttt gggcgtatgc tgggaatgat tctattattg ccaaatcaga 300
aagcaggaga gacccgatga gcgaaatcct agaaacctat tgggcacccc actttggaaa 360
aaccgaagaa gccacagcac tcgtttcata cctggcacaa gcttccggcg atcccattga 420
ggttcacacc ctgttcgggg atttaggttt agacggactc tcgggaaact acaccgacac 480
tgagattgac ggctacggcg acgcattcct gctggttgca gcgctatccg tgttgatggc 540
tgaaaacaaa gcaacaggtg gcgtgaatct gggtgagctt gggggagctg ataaatcgat 600
ccggctgcat gttgaatcca aggagaacac ccaaatcaac accgcattga agtattttgc 660
gctctcccca gaagaccacg cagcagcaga tcgcttcgat gaggatgacc tgtctgagct 720
tgccaacttg agtgaagagc tgcgcggaca gctggactaa ttgtctccca tttaaggagt 780
ccgatttctt tgaatcttac atttcataga gtgagacgct tgcaggttgg ggtttaaacg 840
ttgtggatat cgattccctg caggggagct gtataaagtg tgaggtaaat ctaaaacgca 900
ggacgtgaca tttttggcgc gttttaggtt atactgtctc agacaacgaa actcttgtcc 960
cacattgtga gatttgcttg ctagaatgtg ggctagaaat tcctgaaaat ttttacgcac 1020
tgtaaggacg gtgagttcca tgaccagccc cgtggagaac agcacctcaa ctgagaagct 1080
gaccctggca gagaaggtgt ggcgcgacca tgtcgtgtcc aagggagaaa acggcgagcc 1140
cgacctcctc tacatcgacc tgcagctgct gcatgaagtg acctcaccac aggcattcga 1200
cggcctgcgc atgactggcc gcaaactgcg ccacccagaa ctgcacctgg ccaccgaaga 1260
ccacaacgtg ccaaccgaag gcatcaagac tggctcactg ctggaaatca acgaccagat 1320
ttcccgcctg caggtatcca ccctgcgcga caactgtgaa gagttcggtg ttcgcctgca 1380
cccaatgggt gatgtccgcc agggcatcgt gcacaccgtt ggcccacagc tgggcgcaac 1440
tcagccgggc atgaccattg tgtgcggtga ctcccacacc tctactcacg gcgcgtttgg 1500
ctccatggca ttcggtatcg gtacctctga ggttgagcac gtcatggcca ctcagaccct 1560
gccattgaag cctttcaaga ccatggccat tgaagttact ggcgaactgc agccaggtgt 1620
ttcctccaag gacctgatcc tggcgatcat tgccaagatc ggcaccggtg gtggacaagg 1680
ctacgttctg gaataccgcg gcgaagcaat ccgcaagatg tccatggatg cacgcatgac 1740
catgtgcaac atgtccatcg aagctggcgc acgtgccggc atgatcgccc cagaccaaac 1800
caccttcgac tacgttgaag gccgcgaaat ggcaccaaag ggcgccgact gggacgaagc 1860
agttgcttac tggaagaccc tgccaaccga cgaaggcgca acctttgaca aggtcgtaga 1920
aatcgatggc tccgcactga ccccattcat cacctggggc accaacccag gccaaggtct 1980
gccactgagc gaaaccgtgc caaacccaga agacttcacc aacgacaacg acaaggcagc 2040
agccgaaaag gcactgcagt acatggacct ggtaccagga accccactgc gcgacatcaa 2100
gatcgacacc gtcttcctgg gatcctgcac caacgcccgc atcgaagacc tgcagatcgc 2160
cgctgacatc ctcaagggcc acaaaatcgc cgacggcatg cgcatgatgg tcgtgccttc 2220
ctccatctgg atcaagcaag aggccgaagc actcggactg gacaaaatct tcaccgacgc 2280
tggcgctgaa tggcgtaccg caggctgctc catgtgcctg ggcatgaacc cagaccaact 2340
gaagccaggc gagcgctctg catccacctc caaccgaaac ttcgaaggac gccaaggacc 2400
aggaggccgc acccacctgg tatccccagc agtcgcagcc gccaccgcaa tccgcggcac 2460
cctgtcctca cctgcagata tctaataaat cgactactca catagggtcg ggctagtcat 2520
tctgatcagc gaattccacg ttcacatcgc caattccaga gttcacaacc agattcagca 2580
ttggaccttc tagatcagca ttgtgggcgg tgagatctcc aacatcacag cgcgctgtgc 2640
ccacaccggc ggtacaactt aggctcacgg gcacatcatc gggcagggtg accatgactt 2700
cgccgatccc tgaggtgatt tggatgtttt gttcctgatc caattgggtg aggtggctga 2760
aatcgaggtt catttcaccc acgccagagg tgtagctgct gaggagttca tcgttggtgg 2820
ggatgagatt gacatcgccg attccagggt cgtcttcaaa gtagatggga tcgatatttg 2880
aaataaacag gcctgcgagg gcgctcatga caactccggt accaactaca ccgccgacaa 2940
tccatggcca cacatggcgc tttttctgag gcttttgtgg agggacttgt acatcccagg 3000
tgttgtattg gttttgggca agtggatccc aatgaggcgc ttcgggggtt tgttgcgcga 3060
agggtgcata gtagccctca acgggggtga tagtgcttag atctggttgg ggttgtgggt 3120
agagatcttc gtttttcatg gtggcatcct cagaaacagt gaattcagtg gtgagtagtc 3180
cgcggggtgg aagtggttgt ttcttatgca gggtaccgag ctcgaattcg taatcatggt 3240
catagctg 3248
<210> 7
<211> 1769
<212> DNA
<213> 人工序列(Artificial Sequence)
<400> 7
gcttgcatgc ctgcaggtcg actctagagg atcccctctt tgaatcttac atttcataga 60
gtgagacgct tgcaggttgg ggtttaaacg ttgtggatat cgattccctg caggggagct 120
gtataaagtg tgaggtaaat ctaaaacgca ggacgtgaca tttttggcgc gttttaggtt 180
atactgtctc agacaacgaa actcttgtcc cacattgtga gatttgcttg ctagaatgtg 240
ggctagaaat tcctgaaaat ttttacgcac tgtaaggacg gtgagttcca tgaccagccc 300
cgtggagaac agcacctcaa ctgagaagct gaccctggca gagaaggtgt ggcgcgacca 360
tgtcgtgtcc aagggagaaa acggcgagcc cgacctcctc tacatcgacc tgcagctgct 420
gcatgaagtg acctcaccac aggcattcga cggcctgcgc atgactggcc gcaaactgcg 480
ccacccagaa ctgcacctgg ccaccgaaga ccacaacgtg ccaaccgaag gcatcaagac 540
tggctcactg ctggaaatca acgaccagat ttcccgcctg caggtatcca ccctgcgcga 600
caactgtgaa gagttcggtg ttcgcctgca cccaatgggt gatgtccgcc agggcatcgt 660
gcacaccgtt ggcccacagc tgggcgcaac tcagccgggc atgaccattg tgtgcggtga 720
ctcccacacc tctactcacg gcgcgtttgg ctccatggca ttcggtatcg gtacctctga 780
ggttgagcac gtcatggcca ctcagaccct gccattgaag cctttcaaga ccatggccat 840
tgaagttact ggcgaactgc agccaggtgt ttcctccaag gacctgatcc tggcgatcat 900
tgccaagatc ggcaccggtg gtggacaagg ctacgttctg gaataccgcg gcgaagcaat 960
ccgcaagatg tccatggatg cacgcatgac catgtgcaac atgtccatcg aagctggcgc 1020
acgtgccggc atgatcgccc cagaccaaac caccttcgac tacgttgaag gccgcgaaat 1080
ggcaccaaag ggcgccgact gggacgaagc agttgcttac tggaagaccc tgccaaccga 1140
cgaaggcgca acctttgaca aggtcgtaga aatcgatggc tccgcactga ccccattcat 1200
cacctggggc accaacccag gccaaggtct gccactgagc gaaaccgtgc caaacccaga 1260
agacttcacc aacgacaacg acaaggcagc agccgaaaag gcactgcagt acatggacct 1320
ggtaccagga accccactgc gcgacatcaa gatcgacacc gtcttcctgg gatcctgcac 1380
caacgcccgc atcgaagacc tgcagatcgc cgctgacatc ctcaagggcc acaaaatcgc 1440
cgacggcatg cgcatgatgg tcgtgccttc ctccatctgg atcaagcaag aggccgaagc 1500
actcggactg gacaaaatct tcaccgacgc tggcgctgaa tggcgtaccg caggctgctc 1560
catgtgcctg ggcatgaacc cagaccaact gaagccaggc gagcgctctg catccacctc 1620
caaccgaaac ttcgaaggac gccaaggacc aggaggccgc acccacctgg tatccccagc 1680
agtcgcagcc gccaccgcaa tccgcggcac cctgtcctca cctgcagata tctaagtttt 1740
ggcggatgag agaagatttt cagcctgat 1769
<210> 8
<211> 1448
<212> DNA
<213> 人工序列(Artificial Sequence)
<400> 8
cagtgccaag cttgcatgcc tgcaggtcga ctctagtagg cggcaaaaac gcgcgctgct 60
gaccctgcat ttaaaggcat gcgagtgccc acgggaacca cgttttttag cccggagctg 120
ggctcttggc tggccacaca cgtgcgggtg gtgccggtga ggcgataaag ctgaacggat 180
tcgccggtgc gctccataag gtcggccata attggtacgg ccgtatcgat gagggtgtca 240
gcgccgcgtg cacccaatga ggcaagccgt gcgccgatgg tccatctatt atcgcgggag 300
cgtgccaaca tgccgtgtac ctcaagcgct gaggcgaggc ggtgggctgt agccctgggc 360
agatcggtgg cagctgcgag ctctgccaac gatcgaggct gttctgcgat gacattgagg 420
attaatacag tgcggtctaa aaccttaata ccgctctcgg tggagtcctc gataatttct 480
tgctgtccca ttctttgaat cttacatttc atagagtgag acgcttgcag gttggggttt 540
aaacgttgtg gatatcgatt ccctgcaggg gagctgtata aagtgtgagg taaatctaaa 600
acgcaggacg tgacattttt ggcgcgtttt aggttatact gtctcagaca acgaaactct 660
tgtcccacat tgtgagattt gcttgctaga atgtgggcta gaaattcctg aaaattttta 720
cgcactgtaa ggacggtgag ttccggaagg ctagaaaaag aatggaaaaa tttaccaccc 780
acaccggcgt tggcgttcca ctgcagcgat ccaacgtgga caccgaccag atcatccccg 840
ccgtctacct caagcgcgtc acccgcacag gcttcgaaga cggactgttt tccaactggc 900
gccaaaacga ccccaacttt gtcctcaaca ccgacaccta caagaacggc tccgttctcg 960
tagcaggccc tgactttggc accggctcct cccgcgagca cgccgtctgg gcactcatgg 1020
actacggctt ccgcgctgtc ttctcctcac gattcgccga catcttccgc ggcaactccg 1080
gaaaagctgg catgctcgcc ggcatcatgg aacagtccga catcgaactt ctgtggaagc 1140
tcatggaaca aaccccgggc ctcgaactga ccgtgaacct ggaaaagcag atcgtcactg 1200
caggcgacgt agtgatcagc ttcgaagttg acccttacat tcgctggcgt ttgatggaag 1260
gcctcgacga cgctggcctg accctgcgca agctcgatga aattgaagac tacgaggcta 1320
agcgccctgc gtttaagcca cgcactaacg cttaagtttc agtctgatag cgaaagcacc 1380
ccgcaacctt cattgtcgcg gggtgcattt gggtaccgag ctcgaattcg taatcatggt 1440
catagctg 1448
<210> 9
<211> 2820
<212> DNA
<213> 人工序列(Artificial Sequence)
<400> 9
taggcggcaa aaacgcgcgc tgctgaccct gcatttaaag gcatgcgagt gcccacggga 60
accacgtttt ttagcccgga gctgggctct tggctggcca cacacgtgcg ggtggtgccg 120
gtgaggcgat aaagctgaac ggattcgccg gtgcgctcca taaggtcggc cataattggt 180
acggccgtat cgatgagggt gtcagcgccg cgtgcaccca atgaggcaag ccgtgcgccg 240
atggtccatc tattatcgcg ggagcgtgcc aacatgccgt gtacctcaag cgctgaggcg 300
aggcggtggg ctgtagccct gggcagatcg gtggcagctg cgagctctgc caacgatcga 360
ggctgttctg cgatgacatt gaggattaat acagtgcggt ctaaaacctt aataccgctc 420
tcggtggagt cctcgataat ttcttgctgt cccattcttt gaatcttaca tttcatagag 480
tgagacgctt gcaggttggg gtttaaacgt tgtggatatc gattccctgc aggggagctg 540
tataaagtgt gaggtaaatc taaaacgcag gacgtgacat ttttggcgcg ttttaggtta 600
tactgtctca gacaacgaaa ctcttgtccc acattgtgag atttgcttgc tagaatgtgg 660
gctagaaatt cctgaaaatt tttacgcact gtaaggacgg tgagttccat gaccagcccc 720
gtggagaaca gcacctcaac tgagaagctg accctggcag agaaggtgtg gcgcgaccat 780
gtcgtgtcca agggagaaaa cggcgagccc gacctcctct acatcgacct gcagctgctg 840
catgaagtga cctcaccaca ggcattcgac ggcctgcgca tgactggccg caaactgcgc 900
cacccagaac tgcacctggc caccgaagac cacaacgtgc caaccgaagg catcaagact 960
ggctcactgc tggaaatcaa cgaccagatt tcccgcctgc aggtatccac cctgcgcgac 1020
aactgtgaag agttcggtgt tcgcctgcac ccaatgggtg atgtccgcca gggcatcgtg 1080
cacaccgttg gcccacagct gggcgcaact cagccgggca tgaccattgt gtgcggtgac 1140
tcccacacct ctactcacgg cgcgtttggc tccatggcat tcggtatcgg tacctctgag 1200
gttgagcacg tcatggccac tcagaccctg ccattgaagc ctttcaagac catggccatt 1260
gaagttactg gcgaactgca gccaggtgtt tcctccaagg acctgatcct ggcgatcatt 1320
gccaagatcg gcaccggtgg tggacaaggc tacgttctgg aataccgcgg cgaagcaatc 1380
cgcaagatgt ccatggatgc acgcatgacc atgtgcaaca tgtccatcga agctggcgca 1440
cgtgccggca tgatcgcccc agaccaaacc accttcgact acgttgaagg ccgcgaaatg 1500
gcaccaaagg gcgccgactg ggacgaagca gttgcttact ggaagaccct gccaaccgac 1560
gaaggcgcaa cctttgacaa ggtcgtagaa atcgatggct ccgcactgac cccattcatc 1620
acctggggca ccaacccagg ccaaggtctg ccactgagcg aaaccgtgcc aaacccagaa 1680
gacttcacca acgacaacga caaggcagca gccgaaaagg cactgcagta catggacctg 1740
gtaccaggaa ccccactgcg cgacatcaag atcgacaccg tcttcctggg atcctgcacc 1800
aacgcccgca tcgaagacct gcagatcgcc gctgacatcc tcaagggcca caaaatcgcc 1860
gacggcatgc gcatgatggt cgtgccttcc tccacctgga tcaagcaaga ggccgaagca 1920
ctcggactgg acaaaatctt caccgacgct ggcgctgaat ggcgtaccgc aggctgctcc 1980
atgtgcctgg gcatgaaccc agaccaactg aagccaggcg agcgctctgc atccacctcc 2040
aaccgaaact tcgaaggacg ccaaggacca ggaggccgca cccacctggt atccccagca 2100
gtcgcagccg ccaccgcaat ccgcggcacc ctgtcctcac ctgcagatat ctaaggaagg 2160
ctagaaaaag aatggaaaaa tttaccaccc acaccggcgt tggcgttcca ctgcagcgat 2220
ccaacgtgga caccgaccag atcatccccg ccgtctacct caagcgcgtc acccgcacag 2280
gcttcgaaga cggactgttt tccaactggc gccaaaacga ccccaacttt gtcctcaaca 2340
ccgacaccta caagaacggc tccgttctcg tagcaggccc tgactttggc accggctcct 2400
cccgcgagca cgccgtctgg gcactcatgg actacggctt ccgcgctgtc ttctcctcac 2460
gattcgccga catcttccgc ggcaactccg gaaaagctgg catgctcgcc ggcatcatgg 2520
aacagtccga catcgaactt ctgtggaagc tcatggaaca aaccccgggc ctcgaactga 2580
ccgtgaacct ggaaaagcag atcgtcactg caggcgacgt agtgatcagc ttcgaagttg 2640
acccttacat tcgctggcgt ttgatggaag gcctcgacga cgctggcctg accctgcgca 2700
agctcgatga aattgaagac tacgaggcta agcgccctgc gtttaagcca cgcactaacg 2760
cttaagtttc agtctgatag cgaaagcacc ccgcaacctt cattgtcgcg gggtgcattt 2820
Claims (5)
1.用于抑制YH66-RS07015基因表达的物质的应用,
所述应用为如下(Ⅰ)或(Ⅱ)或(Ⅲ):
(Ⅰ)在提高细菌缬氨酸产量中的应用;
(Ⅱ)在生产缬氨酸中的应用;
(Ⅲ)在提高细菌菌量中的应用;
所述抑制YH66-RS07015基因表达为敲除细菌中的YH66-RS07015基因,
所述细菌为谷氨酸棒杆菌,
所述YH66-RS07015基因为编码YH66-RS07015蛋白的基因,
所述YH66-RS07015蛋白为序列表的序列3所示的蛋白质。
2.一种重组菌,是抑制细菌中的YH66-RS07015基因表达得到的,
所述抑制细菌中的YH66-RS07015基因表达为敲除细菌中的YH66-RS07015基因,
敲除细菌中的YH66-RS07015基因为使细菌基因组DNA中缺失序列表的序列4所示的DNA分子,
所述细菌为谷氨酸棒杆菌。
3.权利要求2所述重组菌在制备缬氨酸中的应用。
4.一种制备缬氨酸的方法,包括如下步骤:发酵权利要求2所述重组菌。
5.一种提高细菌的缬氨酸产量的方法,包括如下步骤:抑制细菌中的YH66-RS07015基因表达,所述抑制YH66-RS07015基因表达为敲除细菌中的YH66-RS07015基因,
所述细菌为谷氨酸棒杆菌,
所述YH66-RS07015基因为权利要求1中所述的YH66-RS07015基因。
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