Day 0 Fix embryos in 4% PFA 5’ wash in PBT __ __ 2’ 100% MeOH __ __ __ __ -20C in MeOH (at least 2hr)
Day 1 5’ in PBT __ __ __ __ ProK (10ug/ml; 1:1000 from 10mg/ml stock) RT __ (no shaking) [1’ for 2-4S; 3’ for 9-13S; 5’ for18-24hpf; 8’-10’ for 30hpf; 20’ for 48hpf; 1hr or longer for >3dpf] Quick PBT wash __ 5’ in PBT __ 20’ 4% PFA RT (30m-1hr) __ 5’ in PBT __ __ __ (split fish into different tubes) 2hr in HYB (RT) at 70C __ O/N (12-18hr) HYB (pre-heated) w/ probe (1:100 from probe stock with 5% dextran sulfate) at 70C __
Day 2 Following at 70C: prewarm solutions, 500ul per tube 5’ 100% HYB __ 5’ 75% HYB:2xSSC __ 5’ 50% HYB:2xSSC __ 5’ 25% HYB:2xSSC __ 5’ 2xSSCT __ 20’ 0.2xSSCT __ 20’ 0.1xSSCT __ __ Following at RT: 500ul per tube 5’ 75% 0.2xSSC:PBT __ 5’ 50% 0.2xSSC:PBT __ 5’ 25% 0.2xSSC:PBT __ 5’ PBT __ Block 2hr in 2mg/ml BSA + 5% sheep serum in PBT (>750ul per tube) on rocker at RT __ O/N at 4C in 150 ul Ab [sheep anti-digoxygenin 1:5000] in blocking solution on shaker __
Day 3 Following at RT on a rocker: Quick wash in PBT __ 25’ PBT (>750ul per tube, shake at RT) __ __ __* 5’ NTMT (400ul/tube) __ __ __ Develop with NBT/BCIP [33.75ul NBT+ 35ul BCIP in 10ml NTMT]: 400ul/tube RT or 32C __ Check after 30m, Stop reaction with PBT 5’ __ __ __ __ (make sure to wash sufficiently) 300ul 25%Glycerol:75%PBS __ 300ul 50%Glycerol:50%PBS __ 300ul 75%Glycerol:25%PBS __ * can be longer
Notes: 50ml NTMT (make fresh, scale it down if necessary): 5ml 1M Tris PH9.5 1ml 5M NaCl 2.5ml 1M MgCl2 250ul 20% Tween20 (or 50ul Tween20) To 50ml with H2O
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How to cite:
Readers should cite both the Bio-protocol preprint and the original research article where this protocol was used:
Huang, P(2019). In situ hybridization protocol. Bio-protocol Preprint. bio-protocol.org/prep119.
Jacobs, C. T. and Huang, P.(2019). Notch signalling maintains Hedgehog responsiveness via a Gli-dependent mechanism during spinal cord patterning in zebrafish. eLife. DOI: 10.7554/eLife.49252
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