Sample preparation

If your cells appear intact with a three-dimensional look to them and there is visible cytoplasm using a phase contrast microscope you could try re-fixing your cells in 1:1 methanol:acetic acid.

Ashley Hart

Business Development Manager, North America

Try pre-fixing your bone marrow or peripheral blood samples by slowly adding ice-cold fix with agitation immediately after the hypotonic treatment to improve your cell preparations.

Graham Halford

FISH Field Application Specialist, Europe

Consider using a mild hypotonic treatment before fixing CD138+ selected cells, which may improve cell morphology.

Laurence Cambridge

FISH Field Application Specialist, Europe

Positively charged slides should only be used for FFPE sections. If these slides are used for cell suspensions, they may produce high green background.

Ashley Hart

Business Development Manager, North America

After pre-treatment, consider using DAPI to assess for over/under digestion of FFPE sections; this can be washed off before applying the FISH probe.

Jenny Morse

FISH Field Application Scientist, North America

When using archived cell pellets, consider re-fixing using fresh fixative to ensure they provide optimal results.

Laurence Cambridge

FISH Field Application Specialist, Europe

Consider using Pepsin to digest excess cytoplasm and cellular debris in Cytospin samples to improve hybridization quality.

Graham Halford

FISH Field Application Specialist, Europe

Try cleaning your slides in 70% ethanol before use, to get rid of any dust or debris. A high degree of debris may lead to a high background.

Jenny Morse

FISH Field Application Scientist, North America

Try to avoid baking or aging of slides (if not needed for another application e.g. G-Banding) as it may reduce signal fluorescence.

Laurence Cambridge

FISH Field Application Specialist, Europe

Perform tissue enzyme digestion at 37°C on a hotplate for best results.

Graham Halford

FISH Field Application Specialist, Europe