Improve Research Reproducibility A Bio-protocol resource
bpdetail_icon_lock
Preprint

Protocol for Nile Red Staining - Fly

JB Jennifer Beck

Last updated date: Mar 27, 2024 Views: 2532

download pdf Download PDF
ask Ask a question
nfavorite Favorite
Procedure

  1. Stock Solution:

    • PBS

    • Fix solution (freshly prepared): 4% paraformaldehyde (PFA) in PBS

    • PBX: PBS, 0.1% Triton X-100

    • Nile Red (500 ul/ml) dissolved in acetone 

  2. Method:

    • Dissect flies in PBS 

    • Fix with 250-300 ul of 4% PFA in PBS for 30 min at room temperature (RT) 

      • 100 mg PFA + 1 ul NaOH + 500 ul H2O --> 20% stock (2-3 min @ 65°C to dissolve) 

      • 50 ul of 20% stock to 200 ul PBS 

    • Wash with 300 ul of PBS for 10 min at RT x3 times. 

    • Incubate with 250 ul of 1 ug/ml Nile Red (0.5 ul NR/sample, 250 ul) in PBX for 2 hrs at RT or overnight at 4°C 

    • Wash with 300 ul of PBX for 5 min at RT x2 times 

    • Incubate with 300 ul of DAPI in PBX (1:4,000 dilution) for 20 min at RT 

    • Wash with 300 ul of PBX for 10 min at RT x3 times 

    • Wash with 300 ul of PBS for 5 min at RT x2 times 

    • Mount on the slide glass with Mowiol medium [M] 

      • align all tissues facing up

      • 1x drop of medium (~35ul]

      • add cover slip

Recipes

Do you have any questions about this protocol?

Post your question to gather feedback from the community. We will also invite the authors of this article to respond.

0/150

tip Tips for asking effective questions

+ Description

Write a detailed description. Include all information that will help others answer your question including experimental processes, conditions, and relevant images.

post Post a Question
0 Q&A
This protocol preprint was submitted via the Bio-protocol Exchange "Submit a Preprint" track.