Agrobacterium tumefaciens mediated explants genetic transformation method

A genetic transformation method and Agrobacterium-mediated technology, applied in the field of Agrobacterium-mediated explant genetic transformation, can solve the problems of inability to suppress, low transformation rate, and high water content of the medium, and achieve the goal of improving transformation efficiency and simplifying preparation. Effect

Inactive Publication Date: 2016-01-13
BEIJING AGRO BIOTECH RES CENT
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Problems solved by technology

[0003] Most of the Agrobacterium cultures are directly cultured by explants on solid medium, because the commonly used medium is added with a large number of elements, trace elements, sucrose and other substances (commonly used co-culture medium components are: MS (mass, trace, organic, Inositol) + 3% (W / V) sucrose + 200uMAS + 0.7% (W / V) agar powder), first, it is easier to infect bacteria; second, due to the high water content of the medium, and there is no filter paper, it is easy to cause Agrobacterium Overgrowth, leading to browning and death of explants due to inability to inhibit the growth of excessive Agrobacterium
When Agrobacterium tumefaciens infects the explants, it is necessary to fully contact the bacterial liquid and the explants so that the T-DNA can be transferred to the plant cells, and the explants must not be too poisoned by Agrobacterium, which will cause the inability to inhibit the explants in the later stage. Excessive Agrobacterium growth browns and kills explants
In the cultivation process of the prior art, the conversion rate is low or even subsequent experiments cannot be carried out due to improper operation of the co-cultivation process.

Method used

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  • Agrobacterium tumefaciens mediated explants genetic transformation method

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Embodiment 1

[0020] A method for Agrobacterium-mediated genetic transformation of explants, comprising: 1) activation of Agrobacterium, 2) Agrobacterium infection of explants and 3) co-cultivation of Agrobacterium and explants, 4) explant induction and Screening and differentiation, the operation of the co-cultivation step of Agrobacterium and explants is: place sterilized Whatman No.1 filter paper on the solid co-culture medium, absorb the bacterial liquid on the surface of the explants after Agrobacterium infection, and place it on Cultivate on the sterile filter paper at 22-23°C for 3-4 days in the dark.

[0021] The preparation method of the solid co-culture medium is as follows: distilled water is added with 0.7% (W / V) agar powder. Add 200 uMAS (acetosyringone) after autoclaving.

[0022] Whatman qualitative filter paper is used in qualitative analysis techniques to identify the properties of substances. Compared with the flat filter paper of the same type, the folded qualitative fi...

Embodiment 2

[0031] This embodiment is a concrete improvement carried out on the basis of embodiment 1

[0032] A method for Agrobacterium-mediated genetic transformation of explants, comprising:

[0033] 1) Activation of Agrobacterium:

[0034] The strain was Agrobacterium EHA105 (pCAMBIA3301). Take out Agrobacterium from -80℃ refrigerator, inoculate in 5ml YEP (add 50mg / L rifampicin (Rif), 5mg / L tetracycline (Tet) and 50mg / L kanamycin (Km)) liquid after thawing on ice In the culture medium, 28°C, 200rpm overnight shaking culture; the next day expanded culture in 50ml YEP liquid medium, shaking culture to OD 600 = 0.6-0.8, collect the bacteria by centrifugation, resuspend in the infection culture medium, add 200 μM acetosyringone before infection to obtain the activated Agrobacterium suspension.

[0035] 2) Agrobacterium-infected explants:

[0036] The explants were selected from Populus montana ( Populus davidiana × P. bolleana ) aseptic seedlings, take fresh and young leaves of as...

Embodiment 3

[0044] A method for Agrobacterium-mediated genetic transformation of explants, comprising:

[0045] 1) Activation of Agrobacterium:

[0046] The Agrobacterium tumefaciens strain was LBA4404, carrying the binary vector plasmid pBI121. The plasmid T-DNA region contains β-glucuronidase (GUS) gene and neomycin phosphotransferase (NPTII) gene, both of which are driven by CaMV35S promoter. Take out the Agrobacterium from the -80°C refrigerator, inoculate it in 5ml YEP (adding 50mg / L rifampicin (Rif), 50mg / L kanamycin (Km)) liquid medium after thawing on ice, 28°C, 200rpm Overnight shaking culture; the next day expanded culture in 50ml YEP liquid medium, shaking culture to OD 600 = 0.6-0.8, collect the bacteria by centrifugation, resuspend in the infection culture medium, add 200 μM acetosyringone before infection to obtain the activated Agrobacterium suspension.

[0047] 2) Agrobacterium-infected explants:

[0048] Common wheat ( Triticum aestivum L.) Young or mature embryos o...

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Abstract

The invneiton discloses an agrobacterium tumefaciens mediated explants genetic transformation method, which comprises agrobacterium activation, agrobacterium infection explants, cocultivation of agrobacterium and explants, induction, screening differentiation of explants, wherein the operations of the cocultivation of the agrobacterium and the explants are that sterilization filter paper is placed on a solid co-culture medium, and a bacterial liquid which is arranged on the surfaces of the explants which are infected by the agrobacterium is placed on the sterilization filter paper to culture for 3-4 days after being sucked clean. A method for preparing the solid co-culture medium is that 0.7% (W / V) agar powder is added into distilled water, and is added with 200 uM acetosyringone after being sterilized in high voltage. The agrobacterium tumefaciens mediated explants genetic transformation method enables the agrobacterium to be capable of fully contacting with the explants not to grow overly when the agrobacterium and the explants are co-cultivated during the genetic transformation process, improves transformation efficiency, and can reduce pollution probability by simplifying culture mediums.

Description

technical field [0001] The invention belongs to the field of transgenic experiment methods, in particular to an agrobacterium-mediated explant genetic transformation method. Background technique [0002] Co-cultivation is the most critical part of the transformation process of plant transgenic experiments. The transfer and integration of T-DNA are completed at this time. After Agrobacterium attaches to the explants, it cannot transform immediately, and the tumor can be induced to go through the "cell regulation period" after 16 hours of attachment, so that T-DNA transfer occurs. Therefore, the co-cultivation time is longer. However, if the co-cultivation time is too long, it may also lead to the excessive proliferation of Agrobacterium, causing the plant cells to be poisoned and die. The proliferation speed of Agrobacterium in co-culture is directly related to the transformation, and the proliferation and growth status of Agrobacterium are related to its infection ability...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N15/84A01H5/00
Inventor 丁莉萍魏建华王宏芝陈亚娟张杰伟李瑞芬
Owner BEIJING AGRO BIOTECH RES CENT
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