生物技术通报 ›› 2026, Vol. 42 ›› Issue (4): 182-189.doi: 10.13560/j.cnki.biotech.bull.1985.2025-0448
董亚茹(
), 聂玉霞, 朱红, 王照红, 刘惠芬, 郭光(
)
收稿日期:2025-04-30
出版日期:2026-04-26
发布日期:2026-04-30
通讯作者:
郭光,男,硕士,研究员,研究方向 :蚕桑综合利用;E-mail: ywk67@126.com作者简介:董亚茹,女,硕士,助理研究员,研究方向 :桑树栽培与育种;E-mail: dongyaru2013@126.com
基金资助:
DONG Ya-ru(
), NIE Yu-xia, ZHU Hong, WANG Zhao-hong, LIU Hui-fen, GUO Guang(
)
Received:2025-04-30
Published:2026-04-26
Online:2026-04-30
摘要:
目的 AP2/ERF家族转录因子是植物特有的调控因子,在植物响应非生物胁迫(如低温、干旱、水涝及高盐)中发挥关键作用。解析桑树ERF转录因子基因MnERF2在干旱胁迫中的分子功能,为桑树抗逆育种提供理论基础和基因资源。 方法 通过花序浸染法获得MnERF2过表达拟南芥株系,分别对转基因幼苗及成苗进行干旱胁迫处理,观测其生长表型,并测定生理生化指标。 结果 过表达MnERF2拟南芥株系失水率比野生型显著降低。干旱胁迫下,过表达幼苗根系发育优于野生型,成苗的生物量积累和叶绿素含量显著提高。此外,干旱胁迫下过表达株系中超氧化物歧化酶(SOD)、过氧化物酶(POD)、过氧化氢酶(CAT)和谷胱甘肽S-转移酶(GST)活性显著增强,抗坏血酸(ASA)、谷胱甘肽(GSH)和脯氨酸含量显著增加,同时显著降低相对电导率及丙二醛(MDA)和活性氧(ROS;O2•-、H2O2、•OH)含量。 结论 MnERF2具有正向调控干旱胁迫响应的功能,过表达MnERF2通过提高植株水分保持能力和生物量,促进脯氨酸生物合成、增加抗氧化酶活性和抗氧化物质含量以提高转基因拟南芥抗旱性。
董亚茹, 聂玉霞, 朱红, 王照红, 刘惠芬, 郭光. 过表达桑树MnERF2增强拟南芥抗旱性[J]. 生物技术通报, 2026, 42(4): 182-189.
DONG Ya-ru, NIE Yu-xia, ZHU Hong, WANG Zhao-hong, LIU Hui-fen, GUO Guang. Overexpression of Mulberry MnERF2 Enhances Resistance to Drought in Arabidopsis thaliana[J]. Biotechnology Bulletin, 2026, 42(4): 182-189.
用途 Application | 引物名称 Primer name | 序列 Sequence (5′‒3′) |
|---|---|---|
PCR验证 PCR verification | pROKⅡ-F | CTATCCTTCGCAAGACCCTTCCTC |
| pROKⅡ-R | GACGTTGTAAAACGACGGCCAGTG | |
实时荧光定量 PCR Quantitative real-time PCR | MnERF2-F | TCCCGTTGGAAGCCGGGA |
| MnERF2-R | CGACAGAGGCGGGACGTT | |
| TUB2-F | GCCAATCCGGTGCTGGTAACA | |
| TUB2-R | CATACCAGATCCAGTTCCTCCTCCC | |
| AtACTIN-F | CCAGCCATCGCTCATCGGAATG | |
| AtACTIN-R | CAGACACTGTATTTTCTCTCTG |
表1 本研究所用引物
Table 1 Primers used in this study
用途 Application | 引物名称 Primer name | 序列 Sequence (5′‒3′) |
|---|---|---|
PCR验证 PCR verification | pROKⅡ-F | CTATCCTTCGCAAGACCCTTCCTC |
| pROKⅡ-R | GACGTTGTAAAACGACGGCCAGTG | |
实时荧光定量 PCR Quantitative real-time PCR | MnERF2-F | TCCCGTTGGAAGCCGGGA |
| MnERF2-R | CGACAGAGGCGGGACGTT | |
| TUB2-F | GCCAATCCGGTGCTGGTAACA | |
| TUB2-R | CATACCAGATCCAGTTCCTCCTCCC | |
| AtACTIN-F | CCAGCCATCGCTCATCGGAATG | |
| AtACTIN-R | CAGACACTGTATTTTCTCTCTG |
图1 过表达MnERF2拟南芥抗性筛选(A)、PCR验证(B)及表达分析(C)M:Marker 2 000;WT:野生型拟南芥;‒:阴性对照;L1‒L5:转化株系。不同小写字母表示差异显著(P<0.05)。下同
Fig. 1 Resistance screening(A), PCR verification(B), and expression analysis (C) of A. thaliana overexpressing MnERF2M: Marker 2 000. WT: Wild-type Arabidopsis thaliana. ‒: Negative control. L1‒L5: Transgenic lines. Different lowercase letters indicate significant differences (P<0.05). The same below
图2 过表达MnERF2拟南芥幼苗的抗旱性评价A:转基因拟南芥和WT植株生长情况(比例尺=1 cm);B:转基因拟南芥和WT植株初生根长;C:转基因拟南芥和WT植株在正常生长条件下失水率
Fig. 2 Evaluation of drought resistance in A. thaliana seedlings overexpressing MnERF2A: The growth of transgenic A. thaliana and WT plants (Scale bar=1 cm). B: Primary root length of transgenic A. thaliana and WT plants. C: Water loss rate of transgenic A. thaliana and WT plants under normal growth conditions
图3 干旱胁迫下过表达MnERF2拟南芥成苗生长特性A:表型(比例尺=1 cm);B:鲜重;C:总叶绿素含量
Fig. 3 Growth characteristics of MnERF2-overexpressing A. thaliana seedlings under drought stressA: Phenotypes (Scale bar=1 cm). B: Fresh weight. C: Total chlorophyll content
图4 干旱胁迫下过表达MnERF2拟南芥相对电导率及MDA含量分析
Fig. 4 Analysis of relative electrolyte leakage and MDA content in MnERF2-overexpressing A. thaliana under drought stress
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