棉花鹽脅迫應(yīng)答基因克隆與功能驗證

發(fā)布時間：2018-05-02 03:21

本文選題：陸地棉 + 鹽脅迫應(yīng)答　；參考：《中國農(nóng)業(yè)大學》2016年博士論文

【摘要】：棉花是鹽堿地先鋒作物。研究耐鹽機理、提高棉花耐鹽性具有重要理論與實踐意義�；趯嶒炇仪捌谘芯抗ぷ�,從鹽脅迫下陸地棉根系抑制性雜交差減文庫篩選得到5個候選基因GhSnRK2.6, GhCIPK6, GhCPK5、GhC2H2和GhWRKY41。通過克隆全長基因,構(gòu)建植物表達載體,分別轉(zhuǎn)化野生型擬南芥及棉花,分析其功能；通過構(gòu)建瞬時表達載體,進行亞細胞定位；通過調(diào)查轉(zhuǎn)基因材料耐鹽相關(guān)性狀,分析這5個鹽脅迫應(yīng)答基因的功能；篩選耐鹽品系,為棉花耐鹽育種提供材料來源。(1)克隆了鹽脅迫應(yīng)答基因GhSnRK2.6, GenBank登錄號為JN872373, ORF全長1,086bp,編碼361個氨基酸。該基因包含9個外顯子,8個內(nèi)含子。構(gòu)建瞬時表達載體p35S-GhSnRK2.6:GFP,基因槍法轉(zhuǎn)化洋蔥表皮細胞進行瞬時表達分析,該蛋白定位于細胞核。構(gòu)建植物表達載體p2301M-GhSnRK2.6,分別轉(zhuǎn)化野生型擬南芥和棉花,分析轉(zhuǎn)基因材料耐鹽性。結(jié)果GhSnRK2.6過表達擬南芥苗期及成熟期的耐鹽性提高；轉(zhuǎn)基因棉花后代材料鹽脅迫下發(fā)芽率顯著高于受體株系,耐鹽性提高；另外,鹽脅迫下轉(zhuǎn)基因棉花的產(chǎn)量性狀和纖維品質(zhì)也優(yōu)于受體對照。(2)構(gòu)建瞬時表達載體p35S-GhCIPK6:GFP,基因槍轟擊法轉(zhuǎn)化洋蔥表皮細胞進行瞬時表達分析,證明GhCIPK6定位于細胞質(zhì)。BiFC分析確定GhCIPK6與GhCBLl和GhCBL8均存在互作關(guān)系,GhCBLl-GhCIPK6復(fù)合體定位于細胞核,GhCBL8-GhCIPK6定位于細胞核及細胞膜。將植物表達載體pBI-GhCIPK6轉(zhuǎn)化棉花,分析耐鹽性。證明鹽脅迫下,GhCIPK6通過參與不同調(diào)控路徑,調(diào)控細胞K+平衡,維持細胞膜穩(wěn)定性,降低鹽脅迫對質(zhì)膜的傷害,保證植株正常生長,提高轉(zhuǎn)基因棉花后代的耐鹽性。(3)構(gòu)建瞬時表達載體進行亞細胞定位,結(jié)果轉(zhuǎn)錄因子GhC2H2定位于細胞核。將前期構(gòu)建的植物表達載體pBI-GhC2H2轉(zhuǎn)化棉花,分析其耐鹽性。結(jié)果證明過表達GhC2H2可提高轉(zhuǎn)基因株系的衣分和單鈴重,促進纖維增長,保證轉(zhuǎn)基因棉花產(chǎn)量,提高轉(zhuǎn)基因棉花后代的耐鹽性。(4)構(gòu)建瞬時表達載體進行亞細胞定位,結(jié)果GhCPK5定位于細胞核。將前期構(gòu)建的植物表達載體pBI-GhCPK5轉(zhuǎn)化棉花,分析相關(guān)性狀,結(jié)果在鹽脅迫下,GhCPK5轉(zhuǎn)基因株系的單鈴重和衣分高于受體,纖維長度增長,馬克隆值下降,斷裂比強度提高,纖維品質(zhì)優(yōu)于受體對照。(5)構(gòu)建瞬時表達載體進行亞細胞定位,結(jié)果轉(zhuǎn)錄因子GhWRKY41定位于細胞核。將前期構(gòu)建的植物表達載體p2301M-GhWRKY41轉(zhuǎn)化棉花并分析耐鹽性。結(jié)果表明,過表達GhWRKY41可提高轉(zhuǎn)基因棉花脅迫下發(fā)芽率,鹽脅迫下轉(zhuǎn)基因株系的鈴重和衣分變化不大,但對纖維品質(zhì)存在不利影響。
[Abstract]:Cotton is a pioneer crop of saline - alkali land . It is of great theoretical and practical significance to study the salt tolerance mechanism and improve the salt tolerance of cotton . Based on the research work in the early stage of the laboratory , five candidate genes GhSnRK2 . 6 , GhCIP6 , GhCP5 , GhC2H2 and GhWRKY41 were isolated from the root system of upland cotton under salt stress .
carrying out sub - cell positioning by constructing a transient expression vector ;
By investigating the salt tolerance properties of transgenic materials , the function of these five salt stress response genes was analyzed .
The expression vector p35S - GhSnR2.6 : GFP was used to transform wild - type Arabidopsis thaliana and cotton to analyze the salt tolerance of transgenic materials .
Under salt stress , the germination rate of transgenic cotton progeny was higher than that of receptor strains , and the salt tolerance was improved .
The results showed that GhCBL8 - GhCBL1 and GhCBL8 could improve the salt tolerance of transgenic cotton . The results showed that GhCBL8 - GhCBL1 was located in the nucleus . The results showed that GhCBL8 - GhCBL8 was located in nucleus .

【學位授予單位】：中國農(nóng)業(yè)大學
【學位級別】：博士
【學位授予年份】：2016
【分類號】：S562
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本文編號：1832165

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棉花鹽脅迫應(yīng)答基因克隆與功能驗證