Method for inducing differentiation of mesenchyma stem cell into islet beta-like cells, and use thereof
A kind of stem cell and cell technology, applied in the field of inducing cell differentiation, can solve the problems of low insulin expression level, unable to achieve clinical application, heavy economic burden, etc., achieve huge economic and social benefits, good plasticity, no tumorigenicity. Effect
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Embodiment 1
[0083] Example 1: Construction of Adxsi-CMV-PDX1 / CMV-NKX6.1 adenoviral vector, the construction method is divided into four steps:
[0084] In the first step, NKX6.1 was excised and connected to the shuttle plasmid vector pShuttle-GFP-CMV (see figure 1 B) (China, Nuosai Genome Research Center Co., Ltd.), obtain pShuttle-GFP-CMV-NKX6.1 (see figure 1 C).
[0085] ①Treatment of shuttle plasmid vector: after combined enzyme digestion with Bgl II+EcoR I (pShuttle-GFP-CMV), dephosphorylation treatment with calf intestinal alkaline phosphatase (Calf Intestinal Alkaline Phosphatase, CIP), after enzyme digestion Add the sample to 1% agarose gel, electrophoresis, cut out the 5.1 kb target fragment of the vector under ultraviolet light, and use the DNA gel recovery and purification kit (column centrifugal type) (for specific steps, refer to the kit instructions, appendix 2. China, Weiglass Biotechnology (Beijing) Co., Ltd., DNA gel recovery and purification kit (column centrifugal type...
Embodiment 2
[0327] Example 2 Isolation, purification, identification and expansion of human fetal liver mesenchymal stem cells:
[0328] 1. Isolation of human fetal liver mesenchymal stem cells
[0329] (1) Isolation, purification and expansion of human fetal liver mesenchymal stem cells: rinse the fetus with sterile normal saline, cut off the umbilical cord, place it in a large beaker, soak it in 75% alcohol for 5 minutes, and remove it from the ultra-clean bench. Take out the fetal liver, wash the blood several times with PBS, cut off the capsule, cut the remaining liver tissue into small pieces, absorb Hank's solution containing 2% FCS with a pointed pipette to wash the liver tissue, collect the liver tissue suspension into 50ml or 15ml aseptic centrifugation In the tube, pipette repeatedly to separate the cells, centrifuge at 50×g for 5 minutes, the pellet is the hepatic parenchymal cells, take the supernatant and transfer it to another centrifuge tube (to remove the hepatic parenchym...
Embodiment 3
[0331] Example 3 Inducing human fetal liver mesenchymal stem cells to differentiate into islet β-like cells:
[0332] Take human fetal liver MSCs (hFL-MSCs) isolated and purified in step Example 2, after the third passage, and reach 80% to 90% fusion, and perform the following three-stage induction to obtain islet β-like cell clusters:
[0333] In the first phase, hFL-MSCs were infected with pAdxsi-CMV-PDX1 / CMV-NKX6.1.
[0334] Transfer cultured mesenchymal stem cells to 75cm 2 Plastic culture flasks to 5 x 10 7 cells / flask; add pAdxsi-CMV-PDX1 / CMV-NKX6.1 virus into the culture flask at an amount of 100PFU / cell, and continue to culture for 4 days; cells transfected with pAdxsi-CMV-GFP empty adenovirus vector simultaneously as negative control In the same group, the expression of EGFP in the cells was observed regularly under the fluorescence microscope. After 24 hours, the cells of each group were lightly washed with PBS, and the cells were fixed with 4% paraformaldehyde or...
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