Primers, probes and kit for detecting leukemia-related fusion genes
A technology of fusion gene and detection primer, which is applied in the field of genetic detection in molecular biology, can solve the problems of limited clinical application, low detection sensitivity, cumbersome and complicated operation, etc., and achieve the effect of good specificity, high sensitivity and simple operation
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Embodiment 1
[0037] Embodiment 1: the extraction of clinical sample RNA
[0038] In this embodiment, RNA is extracted from peripheral blood of leukemia patients and quantified as a template for PCR detection. The RneasyMinikit blood RNA extraction kit provided by Qiagen was used, and the operation was performed according to the instructions, as detailed below:
[0039] a. Add an equal volume of RLT to 0.5-1.5 mL of fresh anticoagulated whole blood sample, vortex or invert gently to mix, and place on ice for 3-5 minutes.
[0040] b. Add an equal volume of absolute ethanol at room temperature and mix well.
[0041] c. Add 700μL to the separation column, centrifuge at 10000rpm for 15s.
[0042] d. Wash the separation column with 700μL of RW1, centrifuge at 10000rpm for 15s.
[0043] e. Rinse the separation column with 500 μL washing liquid RPE, centrifuge at 10000 rpm for 15 s.
[0044] f. Rinse the separation column again with 500 μL washing liquid RPE, centrifuge at 12000 rpm for 2 min....
Embodiment 2
[0047] Example 2: The kit detects the effect of clinical samples
[0048] Leukemia-related fusion gene fluorescent PCR detection kit contains 8 splicing isomers of four common leukemia fusion genes, BCR / ABL, PML / RARα, AML1 / ETO and TEL / AML1. The detection system detects 8 fusion gene splice isoforms sequentially as follows: BCR / ABL (e1a2), BCR / ABL (e13a2), BCR / ABL (e14a2), BCR / ABL (e19a2), PML / RARαL type, PML / RARαS, AML1 / ETO, and TEL / AML1.
[0049] Table 2 Composition of fluorescent PCR detection kit for leukemia-related fusion genes
[0050]
[0051]
[0052] (Note: RT enzyme is reverse transcriptase, which is used to reverse transcribe RNA into cDNA; TaqDNase is DNA polymerase; buffer is reaction buffer; probe is TaqMan-MGB probe)
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