Method for enriching target cells from biology specimen and method for removing leucocyte
A technology for biological samples and leukocytes, applied in the field of enriching target cells and removing leukocytes from biological samples, can solve the problems of high cost, low WBC removal efficiency and time-consuming
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Embodiment 1
[0029] Embodiment 1, the method for removing leukocyte from biological sample
[0030] Dilute human blood in PBS containing 5mM EDTA, add 3 times the volume of RBC lysis buffer (see below for specific components), and gently rotate and shake at room temperature for 12 minutes. The samples were spun at 1500 rpm for 5 minutes to collect the cell pellet. The lysed RBCs in the supernatant were discarded, and the cell pellet was resuspended in 3ml~5ml of PBS containing 5mM EDTA, and passed through anti-CD45 antibody-conjugated Affi-Gel 10 (Pierce, IL, US). and a chromatography column through which the cells were passed in PBS at a flow rate of 2 ml / min to remove WBC, and the flow-through was collected. Compared with utilizing Miltenyi's kit to remove leukocytes in the prior art, the method for removing leukocytes of the present invention significantly reduces cost (the cost of the separation method of the present invention is RMB 80-150 / test; while the cost of Multiny's kit is RMB...
Embodiment 2
[0037] Embodiment 2, the method for enriching target cell from biological sample
[0038] 5ml-10ml of human blood was collected in a test tube containing EDTA and spun at 1500rpm for 3 minutes to pellet RBC and remove plasma including plasma proteins. Dissolve the collected RBC in 10 ml NH-based 4 Cl RBC lysis buffer (specific composition as above) was gently rotated and shaken for 15 minutes. The obtained solution was then spun centrifuged at 1500 rpm for 5 minutes to pellet unlysed cells including WBC and rare cells. The resulting unlysed cell pellet was resuspended in 5 ml PBS, and passed through a 0.5 ml anti-CD45 antibody-coupled Affi-Gel 10 (Pierce, IL, US) affinity chromatography column to remove WBC, wherein the cells were separated in 2 ml / min flow rate in PBS flow through the affinity chromatography column, and collect the flow-through. The collected flow-through containing rare cells was centrifuged at 900g for more than 5 minutes. Cell pellets were resuspended...
Embodiment 3
[0039] Embodiment 3, the yield of the enrichment method of the present invention is verified by admixture research
[0040] Target cells (such as HeLa cells or MCF-7 cells available from ATCC) were prelabeled with 4,6-diamino-2-phenylindole (DAPI) and then spiked into human blood using the method described in Example 1. Methods to enrich spiked cells. The average recovery was about 70% to 80%. Compared with the enrichment method utilizing Miltenyi's kit to remove white blood cells in the prior art, the enrichment method of the present invention significantly reduces cost (the cost of the enrichment method of the present invention is RMB 100-200 / test; while utilizing Multinyi's kit Only the cost of removing white blood cells is RMB 600-700 / test), shortened time (each test of the enrichment method of the present invention needs less than 1 hour to complete the removal of red blood cells and white blood cells; while Multiny's kit only needs to remove white blood cells More than...
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