生物技术通报 ›› 2023, Vol. 39 ›› Issue (11): 226-237.doi: 10.13560/j.cnki.biotech.bull.1985.2023-0417
孙言秋1(
), 谢采芸1,2(), 汤岳琴1,2
收稿日期:2023-04-29
出版日期:2023-11-26
发布日期:2023-12-20
通讯作者:
谢采芸,女,博士,研究方向:酿酒酵母育种;E-mail: xiecy@scu.edu.cn作者简介:孙言秋,女,硕士研究生,研究方向:环境科学与工程;E-mail: sonyeonchu@qq.com
SUN Yan-qiu1(), XIE Cai-yun1,2(), TANG Yue-qin1,2
Received:2023-04-29
Published:2023-11-26
Online:2023-12-20
摘要:
旨在构建优良的高温耐受酿酒酵母菌株,并探究其高温耐受机制。通过CRISPR/Cas9技术在絮凝性工业酿酒酵母KF-7中敲除ASP3(编码 L-天冬酰胺酶II)并进一步高表达CRZ1(编码具有锌指结构的转录因子Crz1p),通过比较转录组解析重组菌株的高温耐受机制。结果显示,在44℃高温条件下,ASP3敲除菌株KAS11利用98.36 g/L葡萄糖产生43.68 g/L乙醇。在KAS11基础上高表达CRZ1后,菌株KASCR7发酵105.37 g/L葡萄糖产48.02 g/L乙醇。与KF-7相比,两个重组菌株的乙醇产量分别提升了4.77%和15.18%。比较转录组分析结果表明,在高温胁迫下,重组菌株的核糖体生物合成及翻译相关基因受到抑制,而热休克蛋白基因以及NAD+、NADH、嘌呤、甘油、脯氨酸等合成相关基因受到诱导,这些响应可能共同导致重组菌株的高温耐受性提升。研究结果可为构建高温耐受酿酒酵母菌株提供优良菌株资源和理论基础。
孙言秋, 谢采芸, 汤岳琴. 耐高温酿酒酵母的构建与高温耐受机制解析[J]. 生物技术通报, 2023, 39(11): 226-237.
SUN Yan-qiu, XIE Cai-yun, TANG Yue-qin. Construction and Mechanism Analysis of High-temperature Resistant Saccharomyces cerevisiae[J]. Biotechnology Bulletin, 2023, 39(11): 226-237.
| 质粒Plasmid | 描述Description | 来源Source |
|---|---|---|
| Cas9-NAT | Ampr; Cas9; NAT1 | [ |
| pMEL13-CRZ1 | Ampr; 2 μm orign, KanMX, gRNA-CRZ1 | [ |
| pMEL13-ASP3 | Ampr; 2 μm orign, KanMX, gRNA-ASP3 | [ |
表1 本研究所用质粒
Table 1 Plasmids used in this study
| 质粒Plasmid | 描述Description | 来源Source |
|---|---|---|
| Cas9-NAT | Ampr; Cas9; NAT1 | [ |
| pMEL13-CRZ1 | Ampr; 2 μm orign, KanMX, gRNA-CRZ1 | [ |
| pMEL13-ASP3 | Ampr; 2 μm orign, KanMX, gRNA-ASP3 | [ |
| 引物用途 Usage of primer | 引物名称Name | 引物序列 Primer sequence(5'-3') |
|---|---|---|
| 扩增带CRZ1同源臂的修复片段 | CRZ1 RF F | GGGCTGAAAAGTACATCCGCGCATTTAACAATTGCTAAGCCACACACCATAGCTTCAAAATG |
| CRZ1 RF R | TAGTCATGTAGGAAGCCATATTTCCGTTGCTGAATGACATTTTGTAATTAAAACT | |
| 高表达CRZ1验证引物 | CRZ1 VP F | GCTTTGACTGCACTTTAGCTTAG |
| CRZ1 VP R | ATTATTACGTCTGTAAGCGC | |
| 敲除ASP3修复片段 | ASP3 RF F | AGAGCAAATGTTGGCTCGCTATTCTTTTGTAAGCAATCTGGTACTCACCAACCTCCAACTAGCCTGATCAGTGACTTTTCATCACACTGTGTTTTTATATAGTTCTTAGTAGTAAATATA |
| ASP3 RF R | TATATTTACTACTAAGAACTATATAAAAACACAGTGTGATGAAAAGTCACTGATCAGGCTAGTTGGAGGTTGGTGAGTACCAGATTGCTTACAAAAGAATAGCGAGCCAACATTTGCTCT | |
| 敲除ASP3验证引物 | ASP3 VP F | TATCAGACCCTTCAGCACGT |
| ASP3 VP R | TGACACTGCTCAAGGGATAA |
表2 本研究所用引物
Table 2 Primers used in this study
| 引物用途 Usage of primer | 引物名称Name | 引物序列 Primer sequence(5'-3') |
|---|---|---|
| 扩增带CRZ1同源臂的修复片段 | CRZ1 RF F | GGGCTGAAAAGTACATCCGCGCATTTAACAATTGCTAAGCCACACACCATAGCTTCAAAATG |
| CRZ1 RF R | TAGTCATGTAGGAAGCCATATTTCCGTTGCTGAATGACATTTTGTAATTAAAACT | |
| 高表达CRZ1验证引物 | CRZ1 VP F | GCTTTGACTGCACTTTAGCTTAG |
| CRZ1 VP R | ATTATTACGTCTGTAAGCGC | |
| 敲除ASP3修复片段 | ASP3 RF F | AGAGCAAATGTTGGCTCGCTATTCTTTTGTAAGCAATCTGGTACTCACCAACCTCCAACTAGCCTGATCAGTGACTTTTCATCACACTGTGTTTTTATATAGTTCTTAGTAGTAAATATA |
| ASP3 RF R | TATATTTACTACTAAGAACTATATAAAAACACAGTGTGATGAAAAGTCACTGATCAGGCTAGTTGGAGGTTGGTGAGTACCAGATTGCTTACAAAAGAATAGCGAGCCAACATTTGCTCT | |
| 敲除ASP3验证引物 | ASP3 VP F | TATCAGACCCTTCAGCACGT |
| ASP3 VP R | TGACACTGCTCAAGGGATAA |
| 培养基Culture medium | 组分Components | pH |
|---|---|---|
| LB+Kana | 5 g/L酵母浸出粉,10 g/L蛋白胨,10 g/L NaCl,0.1 g/L Kana | 7.0 |
| LB+NAT | 5 g/L酵母浸出粉,10 g/L蛋白胨,10 g/L NaCl,0.05 g/L NAT | 7.0 |
| 2% YPD | 10 g/L酵母浸出粉,20 g/L蛋白胨,20 g/L葡萄糖 | 自然 |
| 2% YPD+NAT | 10 g/L酵母浸出粉,20 g/L蛋白胨,20 g/L葡萄糖,0.05 g/L NAT | 自然 |
| 2% YPD+G418 | 10 g/L酵母浸出粉,20 g/L 蛋白胨,20 g/L葡萄糖,0.1 g/L G418 | 自然 |
| 2% YPD+NAT+G418 | 10 g/L酵母浸出粉,20 g/L蛋白胨,20 g/L葡萄糖,0.05 g/L NAT,0.1 g/L G418 | 自然 |
| 5% YPD | 10 g/L酵母浸出粉,20 g/L蛋白胨,50 g/L葡萄糖 | 自然 |
| 15% YPD | 10 g/L酵母浸出粉,20 g/L蛋白胨,150 g/L葡萄糖 | 自然 |
表3 本研究所用培养基
Table 3 Media used in this study
| 培养基Culture medium | 组分Components | pH |
|---|---|---|
| LB+Kana | 5 g/L酵母浸出粉,10 g/L蛋白胨,10 g/L NaCl,0.1 g/L Kana | 7.0 |
| LB+NAT | 5 g/L酵母浸出粉,10 g/L蛋白胨,10 g/L NaCl,0.05 g/L NAT | 7.0 |
| 2% YPD | 10 g/L酵母浸出粉,20 g/L蛋白胨,20 g/L葡萄糖 | 自然 |
| 2% YPD+NAT | 10 g/L酵母浸出粉,20 g/L蛋白胨,20 g/L葡萄糖,0.05 g/L NAT | 自然 |
| 2% YPD+G418 | 10 g/L酵母浸出粉,20 g/L 蛋白胨,20 g/L葡萄糖,0.1 g/L G418 | 自然 |
| 2% YPD+NAT+G418 | 10 g/L酵母浸出粉,20 g/L蛋白胨,20 g/L葡萄糖,0.05 g/L NAT,0.1 g/L G418 | 自然 |
| 5% YPD | 10 g/L酵母浸出粉,20 g/L蛋白胨,50 g/L葡萄糖 | 自然 |
| 15% YPD | 10 g/L酵母浸出粉,20 g/L蛋白胨,150 g/L葡萄糖 | 自然 |
图1 菌株在44℃条件下的发酵结果
Fig. 1 Fermentation result of strains under 44℃
| 菌株 Strain | 乙醇产量 Ethanol production/(g·L-1) | 葡萄糖消耗量 Glucose consumption/(g·L-1) | 乙醇收率Ethanol yield/(g·L-1) | 乙醇产量提升百分比Increased percentage of ethanol production/% |
|---|---|---|---|---|
| KF-7 | 41.69±0.88 | 94.14±2.60 | 0.45±0.02 | / |
| KAS11 | 43.68±0.48* | 98.36±3.28 | 0.44±0.01 | 4.77 |
| KASCR7 | 48.02±1.03** | 105.37±0.89* | 0.46±0.01 | 15.18 |
表4 44℃条件下发酵72 h时各菌株的葡萄糖利用和乙醇生产情况
Table 4 Glucose utilization and ethanol production of each strain after 72 h fermentation at 44℃
| 菌株 Strain | 乙醇产量 Ethanol production/(g·L-1) | 葡萄糖消耗量 Glucose consumption/(g·L-1) | 乙醇收率Ethanol yield/(g·L-1) | 乙醇产量提升百分比Increased percentage of ethanol production/% |
|---|---|---|---|---|
| KF-7 | 41.69±0.88 | 94.14±2.60 | 0.45±0.02 | / |
| KAS11 | 43.68±0.48* | 98.36±3.28 | 0.44±0.01 | 4.77 |
| KASCR7 | 48.02±1.03** | 105.37±0.89* | 0.46±0.01 | 15.18 |
图2 KAS11 vs KF-7和KASCR7 vs KF-7的差异基因火山图
Fig. 2 Volcano plots of DEGs of KAS11 vs KF-7 and KASCR7 vs KF-7
图3 KAS11 vs KF-7和KASCR7 vs KF-7的共有DEGs
Fig. 3 Common DEGs of KAS11 vs KF-7 and KASCR7 vs KF-7
图4 44℃高温胁迫条件下KAS11、KASCR7共同差异基因的KEGG富集分析
Fig. 4 KEGG analysis of common DEGs of KAS11 and KASCR7 under 44℃
| Pathway | Gene | Description | log2 Fold Change | ||
|---|---|---|---|---|---|
| KAS11 vs KF-7 | KASCR7 vs KF-7 | ||||
| Ribosome (P=0.007 65) | RPS22A | Ribosomal 40S subunit protein S22A | -2.12 | -2.43 | |
| RPL11A | Ribosomal 60S subunit protein L11A | -1.82 | -2.39 | ||
| RPS8B | Ribosomal 40S subunit protein S8B | -2.01 | -2.36 | ||
| RPS5 | Ribosomal 40S subunit protein S5 | -1.92 | -2.33 | ||
| RPL12B | Ribosomal 60S subunit protein L12B | -1.96 | -2.31 | ||
| RPL2B | Ribosomal 60S subunit protein L2B | -1.85 | -2.30 | ||
| One carbon pool by folate (P=0.033 83) | ADE17 | Bifunctional Phosphoribosylaminoimidazolecarboxamide formyltransferase/IMP cyclohydrolase | 1.35 | 1.95 | |
| SHM2 | Glycine hydroxymethyltransferase | 1.16 | 2.05 | ||
| GCV1 | Glycine decarboxylase subunit T | 1.59 | 2.15 | ||
| MTD1 | Methylenetetrahydrofolate dehydrogenase(NAD+) | 1.00 | 1.70 | ||
表5 共有DEGs的通路富集结果
Table 5 Enriched pathways of common DEGs
| Pathway | Gene | Description | log2 Fold Change | ||
|---|---|---|---|---|---|
| KAS11 vs KF-7 | KASCR7 vs KF-7 | ||||
| Ribosome (P=0.007 65) | RPS22A | Ribosomal 40S subunit protein S22A | -2.12 | -2.43 | |
| RPL11A | Ribosomal 60S subunit protein L11A | -1.82 | -2.39 | ||
| RPS8B | Ribosomal 40S subunit protein S8B | -2.01 | -2.36 | ||
| RPS5 | Ribosomal 40S subunit protein S5 | -1.92 | -2.33 | ||
| RPL12B | Ribosomal 60S subunit protein L12B | -1.96 | -2.31 | ||
| RPL2B | Ribosomal 60S subunit protein L2B | -1.85 | -2.30 | ||
| One carbon pool by folate (P=0.033 83) | ADE17 | Bifunctional Phosphoribosylaminoimidazolecarboxamide formyltransferase/IMP cyclohydrolase | 1.35 | 1.95 | |
| SHM2 | Glycine hydroxymethyltransferase | 1.16 | 2.05 | ||
| GCV1 | Glycine decarboxylase subunit T | 1.59 | 2.15 | ||
| MTD1 | Methylenetetrahydrofolate dehydrogenase(NAD+) | 1.00 | 1.70 | ||
图5 共有DEGs的蛋白互作网络(PPI)分析
Fig. 5 Protein interaction network analysis for common DEGs
| MCODE | GO/KEGG | Description | P value |
|---|---|---|---|
| MCODE_1 | R-SCE-72706 | GTP hydrolysis and joining of the 60S ribosomal subunit | 1.00×10-100 |
| R-SCE-72689 | Formation of a pool of free 40S subunits | 1.00×10-100 | |
| WP210 | Cytoplasmic ribosomal proteins | 1.00×10-100 | |
| MCODE_2 | WP32 | Translation factors | 6.31×10-8 |
| R-SCE-72662 | Activation of the mRNA upon binding of the cap-binding complex and eIFs, and subsequent binding to 43S | 3.98×10-7 | |
| R-SCE-72649 | Translation initiation complex formation | 3.98×10-7 |
表6 共有DEGs 蛋白互作网络信息
Table 6 Protein interaction network information of common DEGs
| MCODE | GO/KEGG | Description | P value |
|---|---|---|---|
| MCODE_1 | R-SCE-72706 | GTP hydrolysis and joining of the 60S ribosomal subunit | 1.00×10-100 |
| R-SCE-72689 | Formation of a pool of free 40S subunits | 1.00×10-100 | |
| WP210 | Cytoplasmic ribosomal proteins | 1.00×10-100 | |
| MCODE_2 | WP32 | Translation factors | 6.31×10-8 |
| R-SCE-72662 | Activation of the mRNA upon binding of the cap-binding complex and eIFs, and subsequent binding to 43S | 3.98×10-7 | |
| R-SCE-72649 | Translation initiation complex formation | 3.98×10-7 |
图6 44℃高温胁迫条件下KASCR7特有差异基因的KEGG富集分析
Fig. 6 KEGG analysis of common DEGs of KASCR7 under 44℃
| Pathway | Gene | Description | log2 Fold Change |
|---|---|---|---|
| Longevity regulating pathway - multiple species(P=0.008 48) | PNC1 | Nicotinamidase | 1.29 |
| SSA2 | Hsp70 family chaperone | 1.32 | |
| SSA1 | Hsp70 family ATPase | 1.33 | |
| RAS2 | Ras family GTPase | -1.23 | |
| CTT1 | Catalase T | 1.33 | |
| Nicotinate and nicotinamide metabolism(P=0.013 55) | NPT1 | Nicotinate phosphoribosyltransferase | -1.34 |
| PNC1 | Nicotinamidase | 1.29 | |
| NRK1 | Ribosylnicotinamide kinase | 1.44 | |
| SDT1 | Nucleotidase | 1.10 | |
| Biosynthesis of secondary metabolites(P=0.041 39) | PUT1 | Proline dehydrogenase | -1.60 |
| HIS1 | ATP phosphoribosyltransferase | 1.36 | |
| GPD1 | Glycerol-3-phosphate dehydrogenase(NAD+) | 1.60 | |
| TSC13 | Trans-2-enoyl-CoA reductase(NADPH) | -1.52 | |
| TKL2 | Transketolase | 1.29 | |
| CTT1 | Catalase T | 1.33 |
表7 KASCR7 vs KF-7特有DEGs的pathway富集结果
Table 7 Enriched pathways of unique DEGs for KASCR7 vs KF-7
| Pathway | Gene | Description | log2 Fold Change |
|---|---|---|---|
| Longevity regulating pathway - multiple species(P=0.008 48) | PNC1 | Nicotinamidase | 1.29 |
| SSA2 | Hsp70 family chaperone | 1.32 | |
| SSA1 | Hsp70 family ATPase | 1.33 | |
| RAS2 | Ras family GTPase | -1.23 | |
| CTT1 | Catalase T | 1.33 | |
| Nicotinate and nicotinamide metabolism(P=0.013 55) | NPT1 | Nicotinate phosphoribosyltransferase | -1.34 |
| PNC1 | Nicotinamidase | 1.29 | |
| NRK1 | Ribosylnicotinamide kinase | 1.44 | |
| SDT1 | Nucleotidase | 1.10 | |
| Biosynthesis of secondary metabolites(P=0.041 39) | PUT1 | Proline dehydrogenase | -1.60 |
| HIS1 | ATP phosphoribosyltransferase | 1.36 | |
| GPD1 | Glycerol-3-phosphate dehydrogenase(NAD+) | 1.60 | |
| TSC13 | Trans-2-enoyl-CoA reductase(NADPH) | -1.52 | |
| TKL2 | Transketolase | 1.29 | |
| CTT1 | Catalase T | 1.33 |
图7 KASCR7 vs KF-7特有DEGs的蛋白互作网络(PPI)分析
Fig. 7 Protein interaction network analysis for unique DEGs of KASCR7 vs KF-7
| MCODE | GO/KEGG | Description | P value |
|---|---|---|---|
| MCODE_1 | GO:0006913 | Nucleocytoplasmic transport | 7.94×10-5 |
| GO:0051169 | Nuclear transport | 7.94×10-5 | |
| GO:0000055 | Ribosomal large subunit export from nucleus | 7.94×10-5 | |
| MCODE_2 | GO:0019646 | Aerobic electron transport chain | 2.00×10-7 |
| GO:0042773 | ATP synthesis coupled electron transport | 2.00×10-7 | |
| GO:0042775 | Mitochondrial ATP synthesis coupled electron transport | 2.00×10-7 | |
| MCODE_3 | GO:0006364 | rRNA processing | 2.51×10-4 |
| GO:0016072 | rRNA metabolic process | 7.94×10-5 | |
| GO:0042254 | Ribosome biogenesis | 7.94×10-5 | |
| MCODE_4 | GO:0006189 | ‘de novo’ IMP biosynthetic process | 7.94×10-5 |
| GO:0006188 | IMP biosynthetic process | 6.31×10-9 | |
| GO:0046040 | IMP metabolic process | 7.94×10-9 |
表8 KASCR7 vs KF-7特有DEGs蛋白互作网络信息
Table 8 Protein interaction network information for unique DEGs of KASCR7 vs KF-7
| MCODE | GO/KEGG | Description | P value |
|---|---|---|---|
| MCODE_1 | GO:0006913 | Nucleocytoplasmic transport | 7.94×10-5 |
| GO:0051169 | Nuclear transport | 7.94×10-5 | |
| GO:0000055 | Ribosomal large subunit export from nucleus | 7.94×10-5 | |
| MCODE_2 | GO:0019646 | Aerobic electron transport chain | 2.00×10-7 |
| GO:0042773 | ATP synthesis coupled electron transport | 2.00×10-7 | |
| GO:0042775 | Mitochondrial ATP synthesis coupled electron transport | 2.00×10-7 | |
| MCODE_3 | GO:0006364 | rRNA processing | 2.51×10-4 |
| GO:0016072 | rRNA metabolic process | 7.94×10-5 | |
| GO:0042254 | Ribosome biogenesis | 7.94×10-5 | |
| MCODE_4 | GO:0006189 | ‘de novo’ IMP biosynthetic process | 7.94×10-5 |
| GO:0006188 | IMP biosynthetic process | 6.31×10-9 | |
| GO:0046040 | IMP metabolic process | 7.94×10-9 |
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