To help diagnose and classify a leukemia or lymphoma; to help guide treatment; to aid in determining prognosis; to detect and evaluate leukemia or lymphoma cells that remain after treatment or at disease relapse
To help diagnose and classify a leukemia or lymphoma; to help guide treatment; to aid in determining prognosis; to detect and evaluate leukemia or lymphoma cells that remain after treatment or at disease relapse
When you have signs and symptoms that a health care practitioner thinks may be due to leukemia or lymphoma; to help classify the type of leukemia or lymphoma, identify treatment options, and predict the likely course of the disease; to evaluate whether treatment has been effective or detect disease that remains or comes back after treatment (relapse or recurrence)
A blood sample is obtained by inserting a needle into a vein. A bone marrow sample may be collected from the hip bone by a trained health care practitioner (Bone Marrow Aspiration and Biopsy). Sometimes, a tissue sample, such as from a lymph node, is obtained using a biopsy or fine needle aspiration (FNA) procedure. Body fluid samples are obtained through collection of the fluid in a container or by inserting a needle into the body cavity and aspirating a portion of the fluid with a syringe.
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Immunophenotyping by flow cytometry is a laboratory method that detects the presence or absence of white blood cell (WBC) markers called antigens. These antigens are protein structures found on or within WBCs. Specific groupings of these antigens are normally present on or within WBCs and are unique to specific cell types and stages of cell maturation. Additionally, specific patterns of antigens are present on abnormal cells seen in leukemias and lymphomas. Flow cytometry immunophenotyping may be useful in helping to diagnose, classify, treat and determine prognosis of these blood cell cancers.
Leukemias and lymphomas are caused by an abnormal white blood cell that begins to divide uncontrollably, making numerous copies of itself (clones). The abnormal cells grow, but they do not fight infections or perform other functions like normal WBCs. They do not die at a normal rate, so they accumulate in the bone marrow, lymph nodes, or other tissues. As the number of abnormal cells increases in the bone marrow, they may crowd out and inhibit the production of normal white blood cells, red blood cells, and platelets, and eventually abnormal cells may also be released into the blood. As the number of abnormal cells increase in a lymph node, the size of the lymph node increases. Sometimes lymphomas also involve the blood and/or bone marrow.
If you have a leukemia or lymphoma, routine tests such as a complete blood count (CBC) and a WBC differential may show an increased number of white blood cells with a predominance of one type. These tests may suggest lymphoma or leukemia, but more information is generally needed to confirm a diagnosis and to identify a specific type of leukemia or lymphoma.
Flow cytometry immunophenotyping may be performed on blood, bone marrow, or other samples to provide this additional information. It can detect normal cells as well as abnormal cells whose pattern of markers are typically seen with specific types of leukemia and lymphoma. The results may also be used to predict how aggressive the cancer will be and/or whether it will respond to certain treatment.
Most of the antigens that flow cytometry immunophenotyping detects are identified by a CD (clusters of differentiation or cluster designation) number. CD numbers represent a naming convention that is based on international consensus. While hundreds of antigens have been identified and have a unique CD number, only a small number of these are routinely used.
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