Cloning, Expression and Subcellular Localization of DlAGOMEL1 from Longan
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摘要:
目的 探究DlAGOMEL1基因在龙眼体胚发生过程中的调控作用,并明确该基因在亚细胞中的定位,为深入研究DlAGOMEL1基因的功能提供理论依据。 方法 采用RT-PCR技术,基于龙眼基因组数据库,克隆DlAGOMEL1基因的CDS及该基因的5′端上游启动子序列,采用生物信息学方法分析该基因,通过实时荧光定量PCR技术检测其在龙眼体胚不同发育阶段的相对表达量,同时,构建该基因的瞬时融合表达载体,得到重组质粒,并将其瞬时转入洋葱内表皮细胞中,用荧光共聚焦显微镜观察细胞绿色荧光信号。 结果 获得DlAGOMEL1基因CDS全长序列及5′端上游启动子序列长度分别为2655 bp、1512 bp,该基因编码884个氨基酸;系统进化树分析表明,龙眼DlAGOMEL1蛋白与胡杨亲缘关系最近,与单子叶植物水稻、玉米等亲缘关系最远;实时荧光定量分析表明,该基因在龙眼体胚不同阶段均表达,在子叶胚时期(CE)的相对表达量较高,而在球形胚时期(GE)的相对表达量最低。亚细胞定位结果发现,DlAGOMEL1基因定位于细胞质中。 结论 DlAGOMEL1基因在龙眼体胚阶段的相对表达量呈“V”字型,可能主要参与龙眼晚期体胚发生的转录调控过程,在细胞质中发挥主要的功能作用。 -
关键词:
- 龙眼 /
- DlAGOMEL1基因 /
- 表达分析 /
- 亚细胞定位
Abstract:Objective Still unclear regulatory functions of DlAGOMEL1 on the nonembryonic callus and different embryogenic cultures of longan (Dimocarpus longan) were investigated. Method From the longan genome database, the full-length cDNA sequences (CDS) of DlAGOMEL1 and its promoter were obtained using RT-PCR. Bioinformatics of this gene was analyzed and the relative expressions of this gene in embryogenic cultures were detected by real-time quantitative PCR. The recombinant plasmid was constructed from the transient fusion expression vector, and the onion inner epidermal cells transformed into transient onion cells. Green fluorescence signal of the cells was searched under a fluorescence confocal microscope. Result The CDS of DlAGOMEL1 was 2,655 bp which encoded 884 amino acids and the promoter was 1,512 bp. The DlAGOMEL1 of longan and other plants were highly conserved as shown in a multiple sequences analysis. Phylogenetic tree of the protein indicated its close relation with Populars euphonium but not with monocotyledonous plants, such as rice and maize. The gene expressed differently in somatic embryo development stages—most strongly at cotyledon embryo stage and least at spherical embryo stage. The subcellular localization of DlAGOMEL1 was found in cytoplasm. Conclusion Since the relative expression of DlAGOMEL1 was shown to be high at the late stage of longan somatic embryo, the gene might be functionally active in the late stage of the development. The revealed subcellular localization of the gene seemed to predispose its involvement in the cytoplasm of longan. -
Key words:
- Dimocarpus longan /
- DlAGOMEL1 /
- gene expression /
- subcellular localization
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图 1 龙眼DlAGOMEL1基因CDS和启动子序列PCR扩增及融合表达载体的构建
注:(1)M1-DL 2 000 bp,M2-DL 15 kb;(2)A-DlAGOMEL1基因CDS电泳图;B-DlAGOMEL1基因5'端上游启动子序列;C-融合表达载体的pCAMBIA1300-35s-DlAGOMEL1-GFP环状质粒。
Figure 1. Electrophoretograms of CDS of DlAGOMEL1 and promoter by PCR and fusion expression vector in longan
Note: (1) M1-DL 2 000 bp; M2:-DL 15 kb; (2) A-DlAGOMEL1 CDS; B- promoter of DlAGOMEL1; C- fusion expression vector of pCAMBIA1300-35s-DlAGOMEL1-eGFP circular plasmids.
图 5 AGOMEL1蛋白系统发育进化树
Figure 5. Phylogenetic analysis on DIAGOMEL1 from longan and other plants
图 6 龙眼体胚发生不同阶段DlAGOMEL1的相对表达量
注:(1)NEC:非胚性愈伤组织;EC:胚性愈伤组织;ICpEC:不完全胚性紧实结构;GE:球形胚;CE:子叶胚。(2)图中不同小写字母表示差异显著(P<0.05)。
Figure 6. Relative expressions of DlAGOMEL1 at different somatic embryogenesis stages of longan
Note: (1) NEC: Non-embryonic callus; EC: Embryonic callus; ICpEC: Incomplete embryogenic compact structure; GE: Globular embryo; CE: Cotyledon embryo. (2) Different lowercase letters indicate significant differences (P<0.05).
图 7 pCAMBIA1300-35s-DlAGOMEL1-GFP蛋白在洋葱内表皮细胞的亚细胞定位
注:A~C:导入DlLAGOMEL1重组质粒的洋葱内表皮细胞;D~F:导入pCAMBIA1300-35s-GFP空载体的洋葱内表皮细胞;A、D:荧光激发图;B、E:叠加图;C、F:明场图。
Figure 7. Subcellular localization of pCAMBIA1300-35s-DlAGOMEL1-GFP protein in onion
Note: A–C: subcellular locations of endoepidermal cells of onion scale leaf introduced into DlAGOMEL1 recombinant plasmid; D–F: subcellular locations of endoepidermal epidermis cells of onion scale leaf introduced into pcambia1300-35s-GFP empty vector; A and D: flourescent field; B and E: merged field; C and F: bright field.
表 1 引物序列
Table 1. Primer sequence
引物名称
Primer name引物序列
Sequence (5′-3′)用途
Purpose退火温度
Annealing temperature/℃DlAGOMEL1-CF AATATCGACTTCACGCGTCTG 全长验证
Full length validation61 DlAGOMEL1-CQ GCAAGCAACCACAATGAAGC pro-AGOMEL1-F ACTTGTTAGAGACCGACCTAC 启动子克隆
Promoter cloning54 pro-AGOMEL1-R ATACGAGAATCTTGACAATAACC DlAGOMEL1-1300-F CAGTGGTCTCACAACATGACTCGATGCATGATAAG 载体构建
Vector construction61 DlAGOMEL1-1300-R CAGTGGTCTCATACATTCCTGGTGAATAGCATCCA GFP-F AACATACGGAAAACTTACCCT 荧光信号验证
Fluorescence Signal Verification55 GFP-R GTGCAACTCGCTGATCATTAT DlAGOMEL1-QF GGTCTCACTCTCCAAACTCAG 实时荧光定量 PCR
Real-time quantitative PCR58 DlAGOMEL1-QR TTGAAGAAGCAGCTGTCTCC 注:加粗CAGT为保护碱基,下划线为酶切位点。
Note: bold CAGT are the protective bases, and underlined are the restriction sites.
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表 2 龙眼AGOMEL1基因启动子序列顺式作用元件
Table 2. Cis-acting elements of DlAGOMEL1 promoter
顺式元件
Cis element序列
Sequences方向
Strand matrix位置
Position/bp功能
FunctionABRE ACGTG/AACCCGG/CACGTG/ACGTG +/+/−/+ 616/798/1153/1154 脱落酸反应Abscisic acid responsiveness Box 4 ATTAAT − 948 光响应Light responsiveness G-Box CACGTT/CACGTG/GCCACGTGGA −/−/+ 615/1153/1151 光响应Light responsiveness GATA-motif GATAGGA/GATAGGG +/+ 690/1107 光响应Light responsiveness TCT-motif TCTTAC + 212 光响应Light responsiveness CAT-box GCCACT + 1285 分生组织表达Meristem expression LTR CCGAAA + 1353 低温响应Low-temperature responsivenes MBS CAACTG + 1407 参与干旱诱导的MYB结合位点
MYB binding site involved in drought-inducibility注: +: 正向; −: 负向。
Note: +: positive strand; −: negative strand.
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