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HaoKebio? RNA FISH Kit(Animal)

HaoKebio? RNA FISH Kit(Animal)

  • 價(jià)格¥3600
  • 規(guī)格30T
  • 貨號HKR12D
  • 單位
  • 品牌HaoKebio
產(chǎn)品介紹

【Product Information】

Product NameCatalog No30TStorageShelf Life
Wash Buffer (powder, dissolve in 10L ddH2O)HKR12-110LShort-term:4℃Long-term:-20℃12 months
Proteinase K(100x)HKR12-230uL
HRP-Mouse Anti-Digoxin(100x)HKR12-330uL
TSA Chromogenic Solution 570nm (Optional)HKR12-43mL
Blocking BufferHKR12-53mL
Probe:HKR12-63mL
Amplification ProbeHKR12-73mL

【Product Description】

RNA hybridization kit, suitable for in situ hybridization of RNA larger than 300bp, with good specificity and high sensitivity. The reagent kit contains multiple pairs of combination probes. When two probes bind to adjacent positions of the target sequence, a small segment of the top sequence can trigger a branched HCR to form a large molecular nucleic acid aggregate. Each nucleic acid strand is labeled with digoxin, and the antibody recognizes digoxin for color development.

【Tissue Fixation】

Tissue TypeAnimalPlantFrozen SamplesCell Climb SlidesCells
Treatment Fix at RT for 12h, paraffin embedVacuum fix for 1h, RT fix for 12h, paraffin embed.Dehydrate in 15% sucrose at 4℃ for 8h,then in 30% sucrose at 4℃ for 8h, OCT embed.Fix at 4℃ for 2h.scrape off cells,fix in 4% PFA at 4℃ for 2h, wash with PBS, agarose embed.
TypemRNAlncRNAcircRNAmiRNArRNA
TreatmentFix at RT for 12hFix at RT for 12h (<300bp: 24h)Fix at RT for 12hFix at RT for 12hFix at RT for 12h (<300bp: 24h)

【Storage and Shipping】

Ship on wet ice; store at -20℃ for long-term or at 4℃ for short-term use. Shelf life: 6 months.

【Protocol】

1. Deparaffinization and Rehydration

Immerse slides sequentially in:Xylene I (15 min) → Xylene II (15 min) → Xylene III (15 min) → 100% ethanol (10 min) → 90% ethanol (10 min) → 80% ethanol (10 min) → 70% ethanol (10 min) → Rinse with distilled water.

2. Repair

Cell Samples:After the sections are completely dry, use a histology pen (recommended: HKR14P in situ hybridization-specific histology pen) to draw a hydrophobic circle of appropriate size. Place the slides horizontally in an in situ hybridization instrument or a humid chamber. Apply 100 μL of Proteinase K repair solution (1X) onto the tissue and incubate at 37°C for 10 minutes. Rinse with pure water to stop the reaction.

Frozen Sections:For cell samples, after the sections are completely dry, use a histology pen (recommended: HKR14P in situ hybridization-specific histology pen) to draw a hydrophobic circle of appropriate size. Place the slides horizontally in an in situ hybridization instrument or a humid chamber. Apply 100 μL of Proteinase K repair solution (1X) onto the tissue and incubate at 37°C for 20 minutes (for frozen sections). Rinse with pure water to stop the reaction.

Paraffin Sections:Place the slide rack containing the slides into the repair chamber and pour in 1X citrate buffer (pH 6.0) repair solution (ensure the sample area is fully submerged). Cover the chamber, seal it with tape, and place it in a microwave oven. Heat at medium power for 8 minutes, rest for 8 minutes, then heat at medium-low power for another 8 minutes. Allow the solution to cool naturally, then block with 3% hydrogen peroxide for 15 minutes.

3. Blocking

Remove excess liquid from slides. Add 100 μL of Blocking Buffer per slide and incubate at 37℃ for 30 min. Wash once for 5 min.Wash steps: Place slide racks in a wash tank, add wash buffer (ensure samples are submerged), and shake at 60 rpm for 5 min.

4. Probe Hybridization

Remove excess liquid from slides. Add 100 μL of probe per slide and incubate at 37℃ for 3 h or overnight (maintain humidity to prevent drying). Wash 5 times, 5 min each.Wash steps: As described above.

5. Probe Amplification

Remove excess liquid from slides. Add 100 μL of Amplification Probe per slide and incubate at 37℃ for 1.5 h (maintain humidity). Wash 5 times, 5 min each.Wash steps: As described above.

6. HRP-Mouse Anti-Digoxin

Remove excess liquid from slides. Add 100 μL of HRP-Mouse Anti-Digoxin (1X) per slide and incubate at 37℃ in a humidified chamber for 40 min. Wash 5 times, 5 min each. Wash steps: As described above.

7. Chromogenic Reaction

Remove excess liquid from slides. Add 100 μL of TSA Chromogenic Solution per slide and incubate at RT for 10 min. Rinse with distilled water to stop the reaction.

8. DAPI Staining

Add 50 μL of DAPI staining solution per slide, incubate in the dark for 5 min, rinse with distilled water, and mount with anti-fade mounting medium.

【Precautions】

1.Wear lab coats and disposable gloves for safety.

2.For research use only.

【說明書下載】

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