Flow Cytometry
Normal B CD38/10
Loses 10 and 38
Normal B 38 and 20
Loses 38, gains 20 but becomes a bit dimmer at full maturation
Blast gating options
Low SSC, Dim CD45, CD34 Low SSC CD45/SSC usually favored as it will miss less abnormal populations
HLA-DR in monocyte maturation
Maintained. Different than myeloids that lost it early on
CD48,CD117, CD33, CD9, CD68
Mast Cells
CD26
Mature T
When is CD14 acquired by mono line.
Mature monocytes
CD45 + ,CD13 + , CD33 + , CD11b + , CD15 + , CD16 +
Mature neutrophils
How to narrow the coaxial stream? Why would you do so?
Reduce sample stream pressure. Useful when too many cells are passing at once.
Type 2 beads.
Reference beads: Have varying bright fluorescent intensity, can also have antibody binding capacity.
Best B cell lineage markers
CD19,CD79a,CD22,CD10(s)
Easy way to isolated B lymphs from lymph gating.
CD19P CD2N population
Most frequent abberancies in AML
CD2,CD7,CD19,CD56
In what condition do neuts often express CD64
sepsis. be careful when interpreting
ETP Phenotype
+cCD3 + , CD1a - , CD8 - , CD5 dim phenotype, with common co-expression of myeloid antigens (including CD117,CD13 and CD33) and markers of immaturity (i.e. CD34,HLA-DR, TdT and CD133)
Normal K:L Ratio
1:2
Normal RI for hematogones in pediatric marrow
7%~ vs 1-2% in adults
CD9 in ALL
Aberrant when uniform. Usually variable
B cell clonality suspicion when?
Abnormal K:L, weak SIg, aberrant CD5, CD10 e xpression, CD25, CD23, Weak mature B markers, Abberant T markers
Type 1 beads.
Alignment beads: Small beads used for optical alignment.
Other cells found in conventional blast gate
Basos, Monos, early myeloid, hypogranular neuts, dendritic cells
T cells and CD5
Becomes strong while acquiring CD3.
Type 0 beads. Explanation and use.
Blanks: Similar size to lymphocytes but with no added fluorescence. Used for setting thresholds.
Follicular Lymphoma
CD10 positive small cells, pan B with dim CD19. usually CD5 negative.
Alternative for CD34 when looking at myeloid blasts
CD117 or even TdT
Most frequent abberancies in ALL
CD13,CD33,CD15
best monocytic lineage markers
CD14,CD64,CD11c
Markers used to confirm immaturity of T-ALL
CD34,TdT, CD1a, sCD3 lack, HLA-DR lack
Blastic plasmacytoid dendritic cell neoplasm
CD4/CD56/CD103 POS CD34/CD117/MPO/CD64/CD14 NEG
Common megakaryocytic markers?
CD41b,CD42b,CD61
Suspicions for clonal T disorders
CD4:8 abnormal, loss of CD4/CD8 or coexpression, loss of CD7/5, low intensity for T markers, excess of CD2+/CD3- cells. Abberant antigens.
T LGL
CD8+. seen with neutropenia, CD5/CD7 weaker, CD16 pos(strange)
Type 3 beads.
Calibration beads: these beads are equivalent insize to lymphocytes but have varying fluorescence inten-sity, ranging from dim to bright. They share the sameproperties as type IIa, IIb and IIc beads. These beads areused in quantitative flow cytometry where a calibrationcurve is required to determine the antibody bindingcapacity of the cell.
Most common ALL in children
Common > Pre-B > Pro-B
CD34 + , TdT + ,CD19 + , CD10 +
Common ALL immunophenotype
What determines side scatter?
Complexity, granularity of the cell
Doublet exclusion
Doublet exclusion is performed by plotting the height or width against the area for forward scatter or side scatter (Figure 24). Doublets will have double the area and width values of single cells whilst the height is roughly the same. Therefore disproportions between height, width, and area can be used to identify doublets.
CD34 + TdT + CD10 bright CD19 dim CD22 dim CD79b + CD20
Early B precursors
CD34, TdT, DR,CD19 and CD10
Early Hematogones
Sezary syndrome
Expanded CD4 with loss of CD7/CD26 and dim other antigens
Isotype control
Fluorochrome of same class as diagnostic antibody but without any specific affinity
T cell development of CD3
Gained as CD45 increases
HLA-DR in mature T lymphs
Indicates activation. Consider reactive causes
Common cause of CD8 proliferation
Infectious Mono. Other viral lymphocytosis.
Burkitt's Lymphoma
Medium cells with Pan-B and weak SIg, CD10*, TdT Neg. Bright CD45. CD5 neg.
MPO Negative AML. What is the differential
Monoblastic, Erythroid, Mega, Mast Cell, Basophilic, Early AML
When is CD117 usually lost in granulocytes? What about CD34.
Myelocyte stage. CD34 often lost first in pros along with HLA-DR
Use of KIR antibodies
NK neoplasms
CD16
Nk,Neuts
A CD34 + CD117 - CD45 dim CD13 -
Normal B cell precursors
Why are samples warmed to RT?
Optimizes appropriate antibody binding.
Mantle Cell
Pos for most mature b markers including CD5, FMC7, whilst CD10 negative and CD23 negative
T cell development of CD4/8
Precursors negative for both then gain both as thymocytes then develop into one or the other
CD117 in blast populations
Pretty lineage specific to AML, but less so than MPO
CD19 in AML
Pretty rare outside of t(8:21) so quite predictive of such. Often faint positive. Very rarely positive in normal myeloblasts.
TdT in Acute leukemia
Pretty ubiquitous in ALL, sometimes expressed in AML, particularly in early variants
When do monos acquire CD4?
Promonocyte stage where it is brightest
DLBCL
Rare ever present in PB. Often evolves from another disorder. Large cells with strong CD20, FMC7, CD79a, CD22 and CD45 bright. CD10 depends on subtype
CD25 expression in B-ALL
Should prompt investigation of Ph-like BCRABL disease
What determines forward scatter?
Size of the cell
Coexpression of CD34 and bright CD20
Suspicious. Consider Blasts.
CD4
T Helper
CD2
T/NK
CD71
Transferrin marker. Indicates active cells. Not entirely specific to RBC
What beads are usually used for daily QC?
Type 2b.
Which AML most frequently expresses CD2 abberantly
Variant M3
CD38D/CD138B
abnormal plasma cells
CD3 in T-Lymphs
cCD3 gained by precusors, sCD3 only on mature lymphs
When does CD15 appear in grans
later in mature cells
What cell population tend to autofluoresce the most
myeloid due to granules. dead cells.
A CD34 + CD117 + CD45 dim CD13 +
normal mono/myeloid maturing progenitors
CD45d, CD19, CD38b, CD138, restricted cyto Lc, no SIG
plasma cells
best lineage markers for TCell
sCD3, cCD3
Steric hindrance
this is the phenomenon where two antibodies directed at adjacent epitopes can mechanically interfere with each other's binding. This reduced binding results in apparent reduced antigen expression.
CD4:CD8 in HIV
very low
