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Method for expressing and purifying human recombinant interleukin-3

An expression and purification, interleukin technology, applied in the field of expression and purification of human recombinant interleukin-3, can solve the problems of high price, high cost, low yield, etc., and achieve the effect of preventing degradation and reducing load

Active Publication Date: 2011-08-10
GUANGZHOU INST OF BIOMEDICINE & HEALTH CHINESE ACAD OF SCI
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  • Abstract
  • Description
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Problems solved by technology

The expression product of Escherichia coli usually exists in the form of inclusion bodies, and the active form of IL-3 can only be obtained through complex operations of denaturation and renaturation, thereby reducing the yield of active protein; in addition, prokaryotic hosts express especially in Escherichia coli , because of the toxicity caused by the presence of LPS, it is often necessary to analyze and determine the toxicity of the expressed purified product; finally, to obtain a high-purity protein often requires multi-step purification operations, the more purification steps, the higher the protein yield. will be lower and more likely to lead to the inactivation of the target product
Although, insect cells can also express IL-3 protein, but its cost is high and the yield is very low
Therefore, the rhIL-3 recombinant protein currently on the market is extremely expensive

Method used

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  • Method for expressing and purifying human recombinant interleukin-3
  • Method for expressing and purifying human recombinant interleukin-3
  • Method for expressing and purifying human recombinant interleukin-3

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Embodiment Construction

[0029] The Pichia pastoris X-33 strain is selected in the present invention, and the integrated expression plasmid pPICZαA vector is purchased from Invritrogen, USA.

[0030] The medium formula used is as follows:

[0031] 1) Yeast Growth Medium (BMGY):

[0032] Completely dissolve 10g yeast extract, 20g peptone, and dilute to 700mL. Steam autoclave at 121°C for 15-20min, cool to room temperature, add 100mL 1M potassium phosphate solution, 100mL YNB, 2mL 500*B, 100mL 10*GY;

[0033] 2) Yeast induction medium (BMMY)

[0034] Completely dissolve 10g yeast extract, 20g peptone, and dilute to 700mL. Steam autoclave at 121°C for 15-20min, cool to room temperature, add 100mL 1M potassium phosphate solution, 100mL YNB, 2mL500*B, 100mL10*M;

[0035] 3) YPD liquid medium

[0036] Completely dissolve 10g yeast extract, 20g peptone, 10g glucose, dilute to 1000mL, and autoclave at 121℃ for 15-20min. (Solid YPD medium: add 18g agar to YPD liquid medium to obtain YPD solid medium, which is used to p...

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Abstract

The invention discloses a Pichia pastoris transformant capable of expressing human recombinant interleukin-3 (rhIL-3) with high efficiency and a purification method thereof. In the method, the eukaryotic host is pichia pastorisX-33. The purification method comprises the following steps: cloning a human IL-3 gene; establishing a eukaryotic expression vector, and transforming the eukaryotic expression vector into the eukaryotic yeast host; obtaining a yeast transformant for high-level secretory expression by screening, wherein the IL-3 expressed by the yeasts are available in a glycosylated mode and a non-glycosylated module; and performing amplified culture by using a shake flask, and subjecting the supernate of the culture solution to dialysis, nickel affinity purification and further purification by diethylaminoethanol (DEAE) anion column. The purified product is subjected to mass spectrometric identification and analysis, and the result of the mass spectometric identification and analysis indicates that the expressed IL-3 is modified by different glycosyls and that the IL-3 has an his*6 tag and a C-MYC tag and is easy for purification and detection of expression product. In the invention, different from the conventional method using a prokaryotic host to express the rhIL-3, the method for expressing a large amount of rhIL-3 by using a Pichia pastoris expression system is adopted for the first time, quick purification is realized by using a His-tag protein, the purified rhIL-3 is high-activity rhIL-3 protein which is glycosylated to different extents and of which the molecular weight is 19kDa and 22kDa. The method ensures that the high-activity rhIL-3 recombinant protein is obtained quickly.

Description

Technical field [0001] The present invention relates to the application of recombinant DNA technology to produce genetically engineered protein drugs, in particular to an efficient method for expression and purification of human recombinant interleukin-3 (rhIL-3). Background technique [0002] Interleukin 3 (IL-3): also known as multipotent colony stimulating factor (multi-csf), mainly produced by activated cd4+ t cells. Its main function is to promote the directed differentiation and proliferation of pluripotent hematopoietic stem cells in the bone marrow, and to produce various types of blood cells. Because it is not produced in bone marrow stromal cells, it is not often associated with hematopoiesis. It is mainly involved in the body's defense function and is the inflammatory cytokine produced in response. In addition, il-3 can also regulate the growth, differentiation and related gene expression of a variety of mature cells, such as c-myc and il-2r α genes. The molecular we...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N15/24C12N15/81C07K14/54C07K1/22C07K1/18
Inventor 吴东海李洪波金守光徐爱民李侍武
Owner GUANGZHOU INST OF BIOMEDICINE & HEALTH CHINESE ACAD OF SCI
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