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Automated Immunostaining of Cell Smears: An Alternative to Flow Cytometry
  1. Lisa C Happerfield (lh224{at}cam.ac.uk)
  1. Addenbrooke's Hospital, United Kingdom
    1. Rani Saward (rani.saward{at}addenbrookes.nhs.uk)
    1. Addenbrooke's hospital, United Kingdom
      1. Lizz Grimwade (lizz.grimwade{at}addenbrookes.nhs.uk)
      1. Addenbrooke's Hospital, United Kingdom
        1. David Bloxham (david.bloxham{at}addenbrookes.nhs.uk)
        1. Addenbrooke's Hospital, United Kingdom
          1. Wendy N Erber (wendy.erber{at}addenbrookes.nhs.uk)
          1. Addenbrooke's Hospital, United Kingdom

            Abstract

            Aims: A pilot study was performed to assess the applicability of an automated tissue immunostainer machine for the phenotypic anaysis of peripheral blood and bone marrow aspirate smears.

            Methods: Air-dried smears of peripheral blood and bone marrow from normal individuals and 14 cases of haematological malignancies were stained, following fixation, with a range of antibodies to haemopoietic antigens using both immunoperoxidase and immuno-alkaline phosphatase methods on the BondTM-maX (Leica Microsystems) automated immunostaining machine.

            Results: Automated protocols used for staining formalin-fixed paraffin-embedded tissue could be applied to cell smears, giving high quality staining with excellent cytological detail and antigenic preservation for an extensive antibody panel. Optimal quality (morphological preservation and antigen detection without background staining) was obtained with an alkaline phosphatase method and Fast Red chromogenic substrate. Both cell surface and intracellular (cytoplasmic and nuclear) antigens could be detected and gave the expected reactivity.

            Conclusions: Automated immunostaining is possible for haematological smears. It generates consistent high quality staining and is applicable to haematological and, potentially, cytological smears. It provides a practical alternative to flow cytometry and will have particular application when smears are available and there is no suitable sample for flow cytometry.

            • Automation
            • Immunocytochemistry
            • Leukaemia
            • Morphology

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