BCR gene and ABL gene detection probe, preparation method thereof and reagent kit
A gene detection and gene technology, applied in the field of BCR gene and ABL gene detection probes and their preparation, can solve the problems of lack of specificity, high detection kits, etc., achieve good discrimination, good repeatability of results, and improve survival rate Effect
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Embodiment 1B
[0038] The preparation of embodiment 1BCR gene and ABL gene detection probe
[0039]The preparation method of described ABL detection probe (GSPABL), comprises the following steps:
[0040] Clone screening: select clones containing the target gene ABL and both ends of the sequence, such as Figure 1A shown.
[0041] GSPABL1 includes a first probe, a second probe, a third probe, a fourth probe, and a fifth probe, which may be one, several, or a combination of multiples.
[0042] In this embodiment, the combination of five probes was selected, as shown in the following table, which were purchased from Invitrogen RP11BAC and CTDBAC clone libraries.
[0043] ABL1 gene chr9:133,589,268-133,763,062,173,795bp
[0044] Probe set 1
BAC
Insert segment start and end position
3 --> first probe
CTD-2037L19
chr9:133263327…133469440(206Kb)
second probe
RP11-21G10
chr9:133463380…133642562(179Kb)
third probe
CTD-2526G20
chr9:133,...
Embodiment 2
[0061] Embodiment 2: BCR gene and ABL gene detection kit preparation method
[0062] BCR gene and ABL gene detection kit include two components of BCR / ABL hybridization solution and DAPI counterstaining agent, wherein BCR and ABL hybridization solution comprise a group of GSPABL gene probes and two groups of GSPBCR gene probes described in Example 1 combination of needles. The BCR gene has two groups of detection probes, and the ABL gene has a group of detection probes. In the present embodiment, the BCR gene and the ABL gene detection kit are: BCR (group 2+group 3)+ABL (group 1) DAPI counterstaining agents such as combinations, buffer components used in hybridization environment (promoting hybridization), and COTHumanDNA with closed repeat sequences are mainly used for cell counterstaining after hybridization, in which DAPI will bind to DNA, making the cell nucleus appear blue For fluorescence, a counterstain containing p-phenylenediamine can keep the fluorescence stable.
...
Embodiment 3
[0070] Embodiment 3: the detection method of BCR gene and ABL gene detection kit
[0071] 1. Sample processing
[0072] 1.1 Take 2-3ml of peripheral blood or bone marrow to be tested (anticoagulated with sodium heparin) and centrifuge at 2000rpm for 5min, carefully remove the supernatant.
[0073] 1.2 Add 10ml of hypotonic solution (0.075mol / LKCl), mix by pipetting, and let stand for 3min.
[0074] 1.337 ± 1 ℃ water bath box hypotonic 30min.
[0075] 1.4 Add 1ml of fresh fixative, mix by pipetting, and pre-fix at room temperature for 10min.
[0076] 1.5 Mix by pipetting and centrifuge at 2000rpm for 5min.
[0077] 1.6 Remove the supernatant, add 5-10ml of fresh fixative to the sediment, mix by pipetting, and let stand at room temperature for 10min.
[0078] 1. Centrifuge at 72000rpm for 5min, remove the supernatant.
[0079] 1.8 The above washing steps can be repeated until the cell pellet is washed white (this step does not need to stand at room temperature for 10 minute...
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