Molecular marker SIsv0010 closely linked with heading-date gene of millet

A molecular marker and heading date technology, applied in the field of molecular biology, can solve the problem of no literature report on the heading date of millet

Inactive Publication Date: 2011-08-17
深圳华大基因农业控股有限公司
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

At present, rice is more researched on the heading date, but there are basically no literature reports on the research on the heading date of millet

Method used

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  • Molecular marker SIsv0010 closely linked with heading-date gene of millet
  • Molecular marker SIsv0010 closely linked with heading-date gene of millet
  • Molecular marker SIsv0010 closely linked with heading-date gene of millet

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0041] Example 1: Construction of millet F2 generation segregation population

[0042] Male parent: Kangnabujing, high plant type, long and narrow flag leaves, red bristles, red glumes, fertile, greenish leaves, yellow-white pollen, late heading stage. The male parent is Zhang Gu No. 1 seed.

[0043] Female parent: Not resistant to Nabujing, short plant type, short and wide flag leaves, green setae, green glumes, partly sterile, yellowish leaf color, brown pollen, early heading stage. The female parent is the seed of millet A2 male sterile line.

[0044] F2 population construction: male parent and female parent are crossed to obtain F1 generation (the heading stage of F1 is late), and F1 is self-crossed to obtain F2. Among them, F1 is the No. 3 seed of Zhang Zagu. A total of 480 individual plants of the F2 generation were obtained.

[0045] See the Chinese patent application "Molecular marker SIsv0372 closely linked to the herbicide resistance gene of millet", publication ...

Embodiment 2

[0046] Example 2: Extraction of parental and F1 generation, F2 generation individual genomic DNA

[0047] Genomic DNA of the parents, the F1 generation, and 480 F2 generation individuals in Example 1 were extracted by the CTAB method, and the specific methods were as follows:

[0048] (1) Weigh 1.0g of fresh leaves, cut them into pieces and put them in a mortar, grind them with liquid nitrogen, add 3mL 1.5×CTAB, grind them into a homogenate and transfer them to a 15mL centrifuge tube, then add 1mL 1.5×CTAB into the mortar Rinse and transfer to a centrifuge tube. After mixing, place in a water bath at 65°C for 30 minutes, and shake slowly from time to time during this period.

[0049] Among them, the formula of 1.5×CTAB is as follows (1L):

[0050]

[0051] Add deionized water to make up to 1 L, and add mercaptoethanol with a final concentration of 0.2% (2 ml) before use.

[0052] (2) After cooling to room temperature, an equal volume of chloroform / isoamyl alcohol (24:1) ...

Embodiment 3

[0057] Example 3: Preparation of Molecular Markers

[0058] Using the genomic DNA of the male parent, the F1 generation, or the F2 generation extracted in Example 2 as a template, PCR amplification was performed with a pair of molecular marker amplification primers (Seq ID No.2 and Seq ID No.3).

[0059] The PCR reaction system is as follows:

[0060]

[0061]

[0062] The PCR reaction procedure is as follows:

[0063] Pre-denaturation at 94°C for 5 minutes; denaturation at 94°C for 30 seconds, annealing at 60°C for 30 seconds, extension at 72°C for 40 seconds, and 35 cycles; final extension at 72°C for 3 minutes. PCR amplification products can be stored at 4°C.

[0064] Molecular markers are obtained through the above amplification process, and the amplification product is preferably purified after amplification. Sequenced after purification, the result is shown in Seq ID No.1.

[0065] Those skilled in the art can understand that the molecular marker can also be ob...

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Abstract

The invention belongs to the field of molecular biology, and relates to a molecular marker, in particular to a molecular marker closely linked with a heading-date gene of millet. The molecular marker comprises a sequence shown as Seq ID No. 1 (Sequence Identity Number 1). The invention also relates to a primer for amplifying the molecular marker, application of the molecular marker and the primer to heading date gene location of the millet or genetic-breeding of the millet, and a millet breeding method. Through the molecular marker provided by the invention, a genome DNA (Deoxyribonucleic Acid) sequence is linked with the heading-date gene of the millet, so that the establishment of a millet molecular marker assisted breeding system is facilitated; and close genetic linkage distance between the molecular marker and the heading-date gene of the millet is 3.2cM. The molecular marker and the molecular marker amplification primer provided by the invention can be easily, conveniently and rapidly applied to millet breeding practices as well as resource and variety identification at high throughput.

Description

technical field [0001] The invention belongs to the field of molecular biology and relates to a molecular marker, in particular to a molecular marker closely linked with a millet heading date gene. The invention also relates to the primer for amplifying the molecular marker, and the use of the molecular marker and the primer in gene positioning of heading stage of millet or genetic breeding of millet. Background technique [0002] my country is the country of origin of millet (Setaria italica L.Beauv.) and the concentrated planting country of millet in the world. Millet occupies an important position in my country's national economy and social production, and is of great significance to the construction of dry farming ecological agriculture. Therefore, it is particularly important to accelerate the breeding process of millet. Since millet is only a regionally important crop, the current research methods and methods related to millet are relatively backward. How to apply adv...

Claims

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Application Information

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IPC IPC(8): C12N15/11C12N15/63C12N5/10C12Q1/68
Inventor 张耕耘全志武夏秋菊倪雪梅
Owner 深圳华大基因农业控股有限公司
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