In Situ

Protocol for RNA Whole Mount In Situ Hybridization

Contents: Day 0, Day 1, Day 2, Day 3, Day 4, RNA Whole Mount Double In Situ Hybridization, Solutions

♦ DAY 0 - Dehydration

Fixation and Dehydration with MEoH:

• Fixation with 4% PFA was done over night at -40 (maximum).
• In the morning replace to 1% PFA (not a must if you start dehydration straight away).

Dehydration

• PBT 0.1% : 200ml PBSX1 (-/-) with 200ul Tween

Wash PBT	3X5°
25% MEoH	1X5°
50% MEoH	1X5°
75% MEoH	1X5°
100% MEoH	3X5°(in the 3rd time you keep the embryos)

Over night at -20°

♦ DAY 1 - Prehybridization and Hybridization

1.	Rehydration
	75% MeOH/PBT 50% MeOH/PBT 25% MeOH/PBT	1X5° 1X5° 1X5°
2.	Bleaching [optional] - bleach if embryos are stage 19 and up.
	6% H2O2 in PBT for	1 hour. (e.g. 600 ul H2O2 in 10 ml PBT).
3.	PBT	2X5°
4.	Proteinase K	15° (1:1000 in PBT  from 10mg/ml stock)
	17°-18° for big embryos, 10° for small (st. 10) embryos.
5.	Glycine (2 mg/ml in PBT) (Warm for better solubility)	1X10° // stops the proteinase k reaction.
6.	PBT	2X5°
7.	4% PFA +25% Gluteraldehyde (3968ul PBT + 32ul of stock 25%)	1X20°-30°
8.	PBT	Rinse -Pre warm PreHyb to 68°-
9.	PBT	2X5°
10.	50% Prehyb mix/ 50 % PBT	1X10° - Pre-warmed and in bath
11.	PreHyb	>1h - Pre-warmed and in bath
12.	Replace with exactly 2 ml PreHyb and add 5-10 ul of Probe
		O/N at 68° - Pre-warmed and in bath
	(Either Fluorecin or Digoxin labeled probes - amount depends on potency of probe)

Over night at 68° in warm bath

♦ DAY 2 – Post-hybridization washes, blocking, and antibody incubation

1.	Prewarmed Solution X	1X5°	Pre-warmed and in bath
2.	Prewarmed Solution X	4X30°	Pre-warmed and in bath
3.	Prewarmed 50:50 Solution X/MABT	1X10°	Pre-warmed and in bath
4.	MABT	1X5°	RT with shake
	Transfer embryos into net, placed in 6 well. Transfer net to next well each wash
5.	MABT	3X10°
6.	20% goat serum in MABT	>2h
7.	Anti-DIG 1:2000 (or Anti-Fluorecin 1:1500)		O/N at -4° with shake
	(In 20% goat serum in MABT). Cover with aluminium foil.

O/N at -4° with shake

♦ DAY 3: Post-antibody washes

1.	Transfer to RT
2.	MABT	3X10°	RT with shake
3.	MABT	1X1 hour	RT with shake – repeat until going home
4.	Cover with aluminum foil and transfer to O/N shaking at -4°

O/N shaking at -4°

♦ DAY 4: Color development

1.	Transfer to RT
2.	NTMT	3X10°	RT with shake
3.	Reaction mix: BCIP (1:1000) and NBT (1:1000) in NTMT – mix in hood! Allow the reactions to develop at room temperature with gentle rocking. Throughout the development reaction, keep samples covered with aluminum foil to protect them from light and check them periodically to monitor the progress of the reaction.
4.	Stopping the reaction: NTMT	Rinse
5.	TBS-T	3X10°	RT with shake until embryos are clear
	Transfer to a glass vial Replace PBS with PFA 4%, cover in aluminum foil and keep at 4°C.

♦ RNA Whole Mount Double In Situ Hybridization

After color reaction:

1.	TBST	O/N at -4° with shake
2.	PFA 4%	1X30°
3.	TBST	3X 5°
4.	TBST	1X 30° at 65°
5.	TBST	2X 5°
6.	0.1M Glycin-HCl (PH 2.2)	1X 15°
7.	TBST	2X 5°
8.	MABT	2X5°
9.	MABT	2X30°
10.	Blocking (20% Goat Serum in MABT)	2h
11.	Antibody	O/N

O/N at -4° with shake

♦ Solutions:

Pre-hyb  50% formamide (use highest grade – deionized at 40C) 5X SSC, pH 4.5 (use citric acid to pH) 2% SDS  50 mg/ml yeast tRNA 50 mg/ml heparin	for 50 ml 25 ml 12.5 ml // from X20 stock 10 ml // from 10% bottle 250 ul // from sigma 250 ul // from 10 mg/ml stock Complete with DDW-DEPC up to 50 ml
Solution X  50% formamide (below the hood) 2X SSC, pH 4.5 1% SDS	for 50 ml 25 ml 5 ml 5 ml Complete with DDW up to 50 ml
MABT Maleic acid 1M pH 7.5 NaCl Tween 1%	for 200 ml 20 ml 6 ml // from 5M stock 200 ul Complete with DDW up to 200 ml
NTMT NaCl Tris-HCl 2M pH 9.5 MgCl2 Tween 1%	for 200 ml 4 ml // from 5M stock 10 ml // from 20X stock 10 ml // from 1M stock 200 ul Complete with DDW up to 200 ml