Pseudoagglutination – Definition and Clinical Relevance
Pseudoagglutination is a false clumping of red blood cells in laboratory tests that mimics true agglutination but does not involve an immune reaction.
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Pseudoagglutination is a false clumping of red blood cells in laboratory tests that mimics true agglutination but does not involve an immune reaction.
What is Pseudoagglutination?
Pseudoagglutination, most commonly observed as rouleaux formation, is a laboratory phenomenon in which red blood cells (erythrocytes) appear to clump together in a coin-stack or roll-like arrangement. Unlike true agglutination, this process does not involve an antigen-antibody immune reaction. Because it can visually resemble genuine agglutination, pseudoagglutination poses a risk of misinterpretation in blood typing and serological testing.
Causes
Pseudoagglutination results from physical and chemical changes in the blood plasma or in the test medium. Common causes include:
- Elevated plasma proteins: High concentrations of fibrinogen, immunoglobulins, or other proteins reduce the negative surface charge of erythrocytes (zeta potential), causing them to stack together.
- High-molecular-weight additives: Laboratory reagents such as dextran or polyvinylpyrrolidone (PVP) can artificially induce rouleaux formation.
- Cold temperatures: Cold agglutinins can cause reversible, non-immune-mediated clumping at low temperatures.
- Underlying diseases: Conditions such as multiple myeloma, Waldenstrom macroglobulinemia, or chronic inflammatory diseases are associated with elevated plasma proteins that promote rouleaux.
- Sample preparation errors: Contaminated or improperly diluted samples may trigger the phenomenon.
Distinguishing Pseudoagglutination from True Agglutination
Accurate differentiation between true agglutination and pseudoagglutination is essential in transfusion medicine and blood bank serology. Key distinguishing features include:
- Morphology: Pseudoagglutination shows erythrocytes arranged in uniform, stacked rows resembling rolls of coins. True agglutination produces irregular, grape-like clumps.
- Dispersibility: Pseudoagglutinates typically disperse when the sample is diluted with normal saline (0.9% NaCl). True agglutinates remain intact.
- Temperature dependency: Cold-induced pseudoagglutination often resolves when the sample is warmed to 37 degrees Celsius.
Clinical and Diagnostic Relevance
Pseudoagglutination is particularly important in the following medical contexts:
- Blood typing and crossmatching: False positive results can interfere with ABO and Rh blood group determination and pre-transfusion compatibility testing, potentially endangering patient safety.
- Direct antiglobulin test (DAT): Non-specific reactions can mimic hemolytic conditions or autoimmune disorders.
- Hematological evaluation: Prominent rouleaux formation in a peripheral blood smear may indicate elevated protein levels and prompt further investigation for conditions such as multiple myeloma or chronic inflammation.
Management and Laboratory Measures
Pseudoagglutination itself is not a medical condition requiring treatment -- it is a laboratory finding. Appropriate measures include:
- Repeat testing after dilution of the sample with normal saline to disperse the rouleaux.
- Warming the sample to 37 degrees Celsius if cold agglutinins are suspected.
- Using appropriate test media and avoiding high-molecular-weight additives.
- If clinically indicated: investigation of the underlying cause of elevated plasma proteins (e.g., workup for multiple myeloma or inflammatory disease).
References
- Daniels, G. - Human Blood Groups, 3rd Edition, Wiley-Blackwell, 2013.
- World Health Organization (WHO) - Safe Blood and Blood Products: Blood Group Serology, WHO/BLS/93.3.
- Harmening, D.M. - Modern Blood Banking and Transfusion Practices, 6th Edition, F.A. Davis Company, 2012.
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Related search terms: Pseudoagglutination + Pseudo-Agglutination + Pseudoagglutination