生物技术进展 ›› 2026, Vol. 16 ›› Issue (2): 380-387.DOI: 10.19586/j.2095-2341.2025.0100
• 研究论文 • 上一篇
收稿日期:2025-08-06
接受日期:2025-10-22
出版日期:2026-03-25
发布日期:2026-04-27
通讯作者:
咸洪泉
作者简介:王洋 E-mail : wy767466064@163.com基金资助:
Yang WANG(
), Songni YU(
), Yahua LI, Hongquan XIAN(
)
Received:2025-08-06
Accepted:2025-10-22
Online:2026-03-25
Published:2026-04-27
Contact:
Hongquan XIAN
摘要:
黄蓝状菌为菌寄生真菌,其产生的几丁质酶不仅在菌寄生过程中发挥着重要作用,也在植物病害生防和几丁质降解方面具有很高的应用价值。利用PCR技术从黄蓝状菌中克隆出无内含子的几丁质酶基因,采用毕赤酵母表达系统表达几丁质酶,并分析了几丁质酶的特性。结果表明,几丁质酶基因04446、06441开放阅读框大小分别为1 032和1 029 bp,成功构建了毕赤酵母表达载体pPIC9K/04446和pPIC9K/06441,获得高效表达的酵母工程菌株GS115/04446-45和GS115/06441-57;纯化的04446基因表达蛋白Tfch04446为36.8 kD、06441基因表达蛋白Tfch06441为37.2kD。几丁质酶Tfch04446最适反应温度为45 ℃,Tfch06441最适反应温度为50 ℃,且两者最适宜反应pH均为6。Tfch04446的Km为2.27 mg·mL-1,最大反应速度Vmax为0.085 mg·mL-1?min-1,Tfch06441的Km为1.52 mg·mL-1,最大反应速度Vmax为0.067 mg·mL-1?min-1。此外,金属离子Ca2+、Ba2+对几丁质酶Tfch04446活性有促进作用,NH4+有一定的抑制作用;Ba2+对几丁质酶Tfch06441活性有促进作用,Na+、K+、Ca2+、NH4+对其有抑制效果。研究结果可为黄蓝状菌及其几丁质酶的开发及利用奠定基础。
中图分类号:
王洋, 于松尼, 李雅华, 咸洪泉. 黄蓝状菌来源的新型几丁质酶的异源表达及鉴定[J]. 生物技术进展, 2026, 16(2): 380-387.
Yang WANG, Songni YU, Yahua LI, Hongquan XIAN. Heterologous Expression and Characterization of a Novel Chitinase Derived from Talaromyces flavus[J]. Current Biotechnology, 2026, 16(2): 380-387.
| 引物名称 | 序列(5'→3') | 酶切位点类别 |
|---|---|---|
| 04446s | 5'-CGC | AvrⅡ |
| 04446A | 5'-ATTT | NotⅠ |
| 06441S | 5'-G | EcoRⅠ |
| 06441A | 5'-ATTT | NotⅠ |
表1 几丁质酶基因扩增引物
Table 1 Primers for chitinase gene amplification
| 引物名称 | 序列(5'→3') | 酶切位点类别 |
|---|---|---|
| 04446s | 5'-CGC | AvrⅡ |
| 04446A | 5'-ATTT | NotⅠ |
| 06441S | 5'-G | EcoRⅠ |
| 06441A | 5'-ATTT | NotⅠ |
图1 几丁质酶基因04446、06441 PCR扩增产物验证注:M—DL2000 maker;1—几丁质酶基因04446;2—几丁质酶基因06441。
Fig. 1 Verification of PCR amplification products of chitinase genes 04446 and 06441
图2 重组质粒pMD18-T/04446、pMD18-T/06441双酶切产物检测注:M—DL2000 maker;1—AvrⅡ、NotⅠ双酶切pMD18-T/0446;2—EcoRⅠ、NotⅠ双酶切pMD18-T/06441。
Fig. 2 Detection of double digestion products of recombinant plasmids pMD18-T/04446 and pMD18-T/06441
图4 酵母转化子的PCR鉴定A:04446酵母转化子;M—DL5000 marker;1—04446s、04446A为引物的PCR扩增产物;2—5'AOX1、3'AOX1为引物的PCR扩增产物;B:06441酵母转化子;3—06441s、06441A为引物的PCR扩增产物;4—以5'AOX1、3'AOX1为引物的PCR扩增产物
Fig. 4 PCR identification of yeast inverters
图5 几丁质酶Tfch04446、Tfch06441的SDS-PAGE分析注:M—蛋白分子量标准;1—Tfch04446纯化后的蛋白;2—Tfch06441纯化后的蛋白。
Fig. 5 SDS-PAGE analysis of chitinases with Tfch04446 and Tfch06441
| 离子 | 相对活性/% | 离子 | 相对活性/% |
|---|---|---|---|
| H2O | 100.00 | Zn2+ | 0.00 |
| K+ | 95.00 | Ag+ | 102.50 |
| Ca2+ | 144.50 | Mg2+ | 102.20 |
| NH4+ | 51.90 | Ba2+ | 375.00 |
| Mn2+ | 127.00 | Cu2+ | 112.50 |
| Fe2+ | 0.00 | Na+ | 115.00 |
表2 不同离子对Tfch04446活性的影响
Table 2 Effect of different ions on Tfch04446 activity
| 离子 | 相对活性/% | 离子 | 相对活性/% |
|---|---|---|---|
| H2O | 100.00 | Zn2+ | 0.00 |
| K+ | 95.00 | Ag+ | 102.50 |
| Ca2+ | 144.50 | Mg2+ | 102.20 |
| NH4+ | 51.90 | Ba2+ | 375.00 |
| Mn2+ | 127.00 | Cu2+ | 112.50 |
| Fe2+ | 0.00 | Na+ | 115.00 |
| 离子 | 相对活性/% | 离子 | 相对活性/% |
|---|---|---|---|
| H2O | 100.00 | Zn2+ | 0.00 |
| K+ | 53.00 | Ag+ | 123.00 |
| Ca2+ | 53.20 | Mg2+ | 75.00 |
| NH4+ | 59.60 | Ba2+ | 125.00 |
| Mn2+ | 80.90 | Cu2+ | 0.00 |
| Fe2+ | 0.00 | Na+ | 48.00 |
表3 不同离子对Tfch06441活性的影响
Table 3 Effect of different ions on Tfch06441 activity
| 离子 | 相对活性/% | 离子 | 相对活性/% |
|---|---|---|---|
| H2O | 100.00 | Zn2+ | 0.00 |
| K+ | 53.00 | Ag+ | 123.00 |
| Ca2+ | 53.20 | Mg2+ | 75.00 |
| NH4+ | 59.60 | Ba2+ | 125.00 |
| Mn2+ | 80.90 | Cu2+ | 0.00 |
| Fe2+ | 0.00 | Na+ | 48.00 |
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