Bio-Rad VARIANT II HPLC + Sebia Capillarys CZE Hemoglobinopathy Interpreter. Trigger when a user uploads an image of a Bio-Rad VARIANT II HPLC chromatogram (V2_BThal or HbA1c program), a Sebia Capillarys capillary electrophoresis pattern, or both together. Also trigger for: "interpret my Hb electrophoresis", "what does this HPLC show", "interpret my hemoglobin result", "is this thalassemia or iron deficiency", "assess my HbA2/HbF", or any request to correlate hemoglobin fractions with CBC indices for differential diagnosis. Outputs: technology interpretation → fraction analysis → CBC integration → differential diagnosis → condition classification (thalassemia, hemoglobin variant, IDA, ACD, sideroblastic) → confidence scoring → action plan. Asks for missing CBC data before completing diagnosis.
Version: 1.0 | Instruments: Bio-Rad VARIANT II (V2_BThal / V2_HbA1c) · Sebia Capillarys 2/3 OCTA
Standards: ICSH · TIF (Thalassaemia International Federation) · BSH · WHO · ACMG
Brand: EEHLSS / MedLabAI-LIS | Crimson #B71C1C · Navy #0D1B4B · Gold #F9A825
Before interpreting, collect the following. If any item is missing, ask the user before proceeding. Do not generate a diagnosis without at least items 1–4.
Important: HGB in g/L must be converted to g/dL (÷10) for reference range tables. Always confirm units.
(Applied silently during interpretation; reference when explaining an unexpected result)
Technology: Cation-exchange High Performance Liquid Chromatography (CE-HPLC)
Program used: V2_BThal (Beta-Thalassemia Short Program) — 6-minute run
Detection: Absorbance at 415 nm (Soret band of hemoglobin); background correction at 690 nm
How it works:
Bio-Rad V2_BThal Retention Time Windows:
| Window / Peak Name | Retention Time (min) | Normal Hb Expected | Common Abnormal Hb in Window |
|---|---|---|---|
| Unknown (pre-integration) | <1.00 | — | Hb Bart's (γ4), Hb H (β4), bilirubin artefact, acetylated HbF |
| F (HbF) | ~1.10 | <2% adults | ↑ in β-thal, HPFH, δβ-thal, stress erythropoiesis |
| Unknown | ~1.21 | — | Various minor peaks; inspect chromatogram |
| P2 | ~1.33 | <4% | Post-translational HbA0 modification; degradation product |
| P3 | ~1.71 | <4% | Modified HbA0; also seen with HbH/Bart's; α-thal marker |
| Ao (HbA) | ~2.43 | 95–98% adults | Low in all hemoglobin disorders |
| A2 (HbA2) | ~3.65 | 2.0–3.3% | ↑β-thal trait (>3.5%); ↓IDA; co-elutes with HbE, HbC (false ↑) |
| S-window | ~4.41 | 0% | HbS; also Hb D-Punjab, Hb G-Coushata (same window, different RT) |
| C-window | ~5.10 | 0% | HbC; also Hb O-Arab, Hb E (HbE usually earlier in HPLC — see note) |
| D-window | ~4.05–4.30 | 0% | Hb D-Punjab, Hb G-Coushatta |
Critical HPLC Interpretation Rules:
A2 Calibrated vs. Area %:
* = outside expected ranges (instrument flag — not necessarily pathological; interpret in context)Technology: Capillary Zone Electrophoresis (CZE) in free solution
Detection: Direct absorbance at 415 nm
How it works:
Sebia CZE Zone Map (Capillarys 2/3):
| Zone | Position | Normal Hb / Common Variants |
|---|---|---|
| Z1 | Far right | HbA2', Hb Hope, fast variants |
| Z2 | Rare variants | |
| Z3 | Rare variants | |
| Z4 | Hb J Baltimore, Hb J Oxford | |
| Z5 | HbS (diagnostic position) | |
| Z6 | Hb D-Punjab, Hb G variants (co-migrate with S in HPLC but separable here) | |
| Z7 | Hb Lepore (β/δ fusion), Hb G-Philadelphia | |
| Z8 | HbF (fetal hemoglobin) | |
| Z(A) = Z9 | Centre | HbA (anchor zone) — always the largest peak in normal adult |
| Z10 / Z(A) area | HbA (shaded/filled peak) | |
| Z(F) | HbF (when elevated) | |
| Z(D) | HbD-Punjab zone | |
| Z(S) | HbS zone | |
| Z(E) | HbE zone (unlike HPLC, CZE separates HbE from HbA2) | |
| Z(A2) | ~position 235–245 | HbA2 (separated from HbE and HbC on CZE) |
| Z(C) | Far left | HbC — "Hb C or Hb variant" label |
| Z14, Z15 | Leftmost | Slow variants; Hb H suspected if wide fraction 0.3–32% in Z15; Hb Bart's in Z12 |
Critical CZE Interpretation Rules:
| Fraction | HPLC (Bio-Rad V2_BThal) | CZE (Sebia Capillarys) | Significance if Outside Range |
|---|---|---|---|
| HbA | 95.0–97.5% | 95.0–98.0% | Low in all hemoglobin disorders |
| HbA2 | 2.0–3.3% | 1.6–3.1% (note higher CZE values) | >3.5% HPLC / >3.2% CZE → β-thal trait |
| HbF | <2.0% | <2.0% | >2% → HPFH, δβ-thal, β-thal; stress erythropoiesis |
| HbS | 0% | 0% | Present → sickle cell trait (35–45%) or disease (>80%) |
| HbC | 0% | 0% | Present → HbC trait (~40%) or disease |
| HbE | 0% | 0% | Present → HbE trait, disease, or HbEβ-thal |
| HbD-Punjab | 0% | 0% | Present → HbD trait; S-window HPLC — distinguish by CZE/sickling |
| HbH | 0% | 0% | Present → α-thalassemia (Hb H disease: 3-gene deletion) |
| Hb Bart's | 0% | 0% | Present → α-thalassemia; Hb Bart's hydrops fetalis (4-gene del) |
Elevated HbA2 (>3.5% HPLC / >3.2% CZE) — Rule Out List:
| HbA2 Value (HPLC) | Likely Diagnosis | Supporting CBC | Action |
|---|---|---|---|
| 3.5–7.0% | β-thalassemia trait | MCV <75, MCH <27, normal/low RBC, low Hb | Confirm by CZE; family study |
| 3.5–7.0% | β-thal trait + iron deficiency | MCV low, ferritin low | Treat IDA first, recheck HbA2 |
| >10% on HPLC | HbE co-elution | MCV low-normal, target cells on film | CZE mandatory to separate |
| >10% on CZE | Hb Lepore or HbE co-migration | — | HPLC correlation; molecular |
| 5–8% | Possible HbC/HbO-Arab co-migration with A2 | — | C-window check; CZE |
| 5–8% | Hb Lepore trait | Microcytic; Lepore RT ~3.46 min | CZE/electrophoresis |
Low HbA2 (<2.0% HPLC / <1.6% CZE) — Rule Out List:
| Scenario | Likely Cause |
|---|---|
| Low HbA2 + microcytic hypochromic anemia | Iron deficiency — IDA suppresses HbA2 production; treat IDA and retest |
| Low HbA2 + microcytosis + normal iron | δ-thalassemia; Hb H disease |
| Low HbA2 + normal CBC | Normal variant; some ethnic groups; sideroblastic anemia |
Step 1: Classify anemia if present
Step 2: Microcytic Anemia Differential — Discriminant Indices
Apply these indices to distinguish the major causes of microcytic anemia:
| Index | Formula | β-thal Trait | IDA | ACD | Sideroblastic |
|---|---|---|---|---|---|
| Mentzer Index | MCV ÷ RBC | <13 → thal | >13 → IDA | Variable | Variable |
| England & Fraser | MCV − RBC − (5×HGB) − 3.4 | <0 → thal | >0 → IDA | — | — |
| Green & King (GK) Index | MCV² × RDW ÷ (HGB × 100) | <65 → thal | >65 → IDA | — | — |
| RBC Morphology Index (RDWI) | MCV × RDW ÷ RBC | <220 → thal | >220 → IDA | — | — |
| Shine & Lal | MCV² × MCH ÷ 100 | <1530 → thal | >1530 → IDA | — | — |
These indices are screening tools only — none has 100% sensitivity/specificity. Always combine with Hb studies and iron parameters.
Step 3: Typical CBC Profiles by Condition
| Parameter | β-thal Trait | α-thal Trait (1–2 gene del) | IDA | ACD | Sideroblastic | HbE Trait | HbS Trait |
|---|---|---|---|---|---|---|---|
| HGB | Mildly low or N | Mildly low or N | Low | Low-mod | Low | N or slightly low | Usually N |
| MCV | Low (<75 fL) | Low-normal (70–80) | Low | N-low | Low-normal | Low (60–75 fL) | N |
| MCH | Low | Low-normal | Low | N-low | Low | Low | N |
| MCHC | N-low | N | Low | N | Variable | N-low | N |
| RDW | N or mildly ↑ | N | Markedly ↑ | N | ↑ (dimorphic) | N | N |
| RBC count | N or ↑ | N or ↑ | ↓ | ↓ | ↓ | N | N |
| Ferritin | N | N | ↓↓ | ↑ or N | ↑ or N | N | N |
| Serum Iron | N | N | ↓↓ | ↓ | ↑ or N | N | N |
| TIBC | N | N | ↑↑ | ↓ or N | N | N | N |
| Trf Sat | N | N | <15% | <20% | ↑ or N | N | N |
| HbA2 | >3.5% | N or low | Low-N | N-low | N | High (co-elutes on HPLC) | N |
| HbF | N or ↑1–5% | N | N | N | N | N | N |
This is the most clinically important differential at the CBC level. Both present with microcytic hypochromic picture.
Favours IDA over β-thalassemia trait:
Favours β-thalassemia trait over IDA:
Compound β-thal trait + IDA (IMPORTANT):
| Feature | Finding in ACD |
|---|---|
| HGB | Mild-moderate reduction (90–120 g/L / 9–12 g/dL) |
| MCV | Normal or mildly low (normocytic or mildly microcytic) |
| RDW | Usually normal |
| Ferritin | Normal or ELEVATED (ferritin is acute phase reactant) |
| Serum iron | Low |
| TIBC | Low or normal (unlike IDA where TIBC is high) |
| Transferrin saturation | Low |
| Hepcidin | Elevated (not routinely measured but underlying mechanism) |
| Reticulocyte | Inappropriately low for degree of anemia |
| Clinical context | Active chronic illness: infection (TB, HIV, malaria), autoimmune disease, cancer, CKD |
ACD vs IDA (when TIBC not available):
| Feature | Sideroblastic Anemia |
|---|---|
| CBC | Microcytic or normocytic anemia; often dimorphic RBC population on film |
| RDW | Elevated (dimorphic) |
| MCV | Variable (can be low, normal, or high in congenital form) |
| Serum iron | Elevated or normal |
| Ferritin | Elevated |
| TIBC | Normal or low |
| Transferrin saturation | Elevated |
| Hb studies | Usually normal HbA2/HbF; no hemoglobin variant |
| Film | Hypochromic microcytes + normochromic cells = dimorphic; Pappenheimer bodies |
| Bone marrow | Ring sideroblasts on Prussian blue stain (>15% = WHO criteria for refractory anemia with ring sideroblasts) |
| Causes | Congenital (X-linked ALAS2 mutation); acquired: alcohol, lead, drugs (isoniazid, chloramphenicol, pyrazinamide), MDS |
| Key clue | High ferritin/serum iron + microcytic/dimorphic anemia + normal Hb fractions |
Step 1: Do the HbA2 values agree (after method adjustment)?
Step 2: Does CZE identify a variant that HPLC placed in a shared window?
Step 3: Quantitative comparison of HbA percentage
Step 4: HbF assessment
| Genotype | HbA2 | HbF | HbA | HbS/C/E | CBC | Diagnosis |
|---|---|---|---|---|---|---|
| β-thal trait (β/β+) | >3.5% (HPLC) | N or ↑1–5% | ↓ slightly | 0% | Microcytic, normal RBC count | β-thalassemia carrier — does NOT cause significant clinical disease |
| β-thal intermedia | >3.5–5% | 20–40% | ↓↓ | 0% | Moderate anemia, microcytic | Significant disease; transfusion-independent mostly |
| β-thalassemia major (β0/β0) | Unmeasurable | 80–100% | 0% | 0% | Severe anemia; transfusion dependent | Cooley's anemia |
| δβ-thal trait | Low/normal A2 | ↑ (5–20%) | ↓ | 0% | Microcytic | δβ-thalassemia; A2 not elevated |
| HPFH | Low A2 | ↑↑ (15–30% het) | ↓ but less so | 0% | Normal or mild anemia | Hereditary persistence of HbF — often benign |
| Genotype | HbA2 | HbF | HbA | Hb Bart's / HbH | CBC | Diagnosis |
|---|---|---|---|---|---|---|
| Silent carrier (--/αα) | N | N | N | 0–1% Bart's neonatal | Normal | Asymptomatic; may pass on to child |
| α-thal trait (--/αα or -α/-α) | Low-N | N | N | 0% adults | Mild microcytosis, normal Hb | α-thalassemia trait |
| Hb H disease (--/-α) | Low | N | ↓ | HbH 5–30% | Moderate microcytic anemia | Significant hemolysis; splenomegaly |
| Hb Bart's hydrops (-α/--) neonatal | — | — | 0% | Bart's >80% | Hydrops fetalis | Incompatible with life without intervention |
| P3 elevation on HPLC | Low-N | N | N | 0% | Mild microcytosis | Suggestive of α-thalassemia — α-globin gene analysis recommended |
| Variant | HPLC Findings | CZE Findings | CBC Typical | Clinical |
|---|---|---|---|---|
| HbS trait | S-window 35–45%, HbA 55–60% | Z5 ~35–45% | Normal usually | Asymptomatic; sickling under extreme hypoxia |
| HbSS (sickle cell disease) | S-window >80%, HbA 0%, HbF variable | Z5 >80%, no HbA | Low HGB, high MCV (hemolysis), high bilirubin | Vaso-occlusive crises, hemolytic anemia, multi-organ |
| HbSβ-thalassemia | HbS 60–80%, HbA 0–20%, HbA2 >3.5% | S in Z5, elevated A2 | Microcytic anemia | Variable severity by β0 or β+ mutation |
| HbC trait | C-window 35–45%, HbA 55–60% | Z(C) ~35–45% | Normal CBC | Asymptomatic |
| HbCC disease | C-window >90%, HbA 0% | Z(C) dominant | Mild anemia, microcytic | Mild hemolytic anemia; splenomegaly |
| HbE trait | HPLC: apparent HbA2 ~25–30% (HbE+A2 co-elution), HbA 65–75% | CZE: HbE in Z(E) ~25–30%, HbA2 separate ~2–3% | Mild microcytosis; MCV 65–80 fL | Asymptomatic |
| HbEβ-thalassemia | HPLC: HbE+HbA2 co-elution, HbF elevated, HbA low | CZE: HbE >50%, HbF elevated, HbA low | Significant microcytic anemia | Clinically variable; can mimic β-thal major |
| HbD-Punjab | S-window on HPLC, ~35–45%, HbA 55–60% | Z6 (NOT Z5) — differentiates from HbS | Normal or mild | Sickling test NEGATIVE — key distinction from HbS |
| HbH disease | P3 elevation, possible pre-integration Hb H peak | Z15 wide fraction ("Hb H suspected") | Moderate anemia, microcytic | Hemolytic; Heinz bodies on film; splenomegaly |
Use this structured format for every interpretation:
Patient: Age ___ | Sex ___ | Sample ID: ___
Instruments: [Bio-Rad VARIANT II HPLC V2_BThal] + [Sebia Capillarys CZE] | Date: ___
Clinical Context: ___
| Fraction | HPLC Result | HPLC Reference | CZE Result | CZE Reference | Status | Notes |
|---|---|---|---|---|---|---|
| HbA | X% | 95–97.5% | X% | 95–98% | ✅/⚠️/🚨 | |
| HbA2 | X% | 2.0–3.3% | X% | 1.6–3.1% | ||
| HbF | X% | <2% | X% | <2% | ||
| HbS / variant | X% | 0% | X% | 0% | ||
| Unknown peaks | Describe RT + % | — | Zone + % | — |
| Parameter | Result | Reference (Age/Sex) | Status | Interpretation |
|---|---|---|---|---|
| HGB | X g/dL | X–X | ✅/⬇️/🚨 | |
| RBC | X ×10⁶/µL | X–X | ||
| HCT | X% | X–X | ||
| MCV | X fL | 80–100 | ||
| MCH | X pg | 27–33 | ||
| MCHC | X g/dL | 32–36 | ||
| RDW-CV | X% | 11.5–14.5 |
Discriminant Index Results:
| Index | Calculated Value | Cut-off | Interpretation |
|---|---|---|---|
| Mentzer Index (MCV÷RBC) | X | <13=thal; >13=IDA | |
| England & Fraser | X | <0=thal; >0=IDA | |
| Green & King | X | <65=thal; >65=IDA | |
| Shine & Lal | X | <1530=thal; >1530=IDA | |
| RDWI | X | <220=thal; >220=IDA |
Overall Index Consensus: [e.g., "4 of 5 indices favour β-thalassemia trait"]
HPLC Chromatogram:
CZE Electrophoretogram:
Primary diagnosis: [Most likely condition with evidence]
Confidence level: High / Moderate / Low
Evidence supporting:
Alternative diagnoses to exclude:
Conditions EXCLUDED by these results:
(Complete only when iron data available; otherwise note as pending)
| Parameter | Result | Reference | Status | Interpretation |
|---|---|---|---|---|
| Serum Ferritin | X µg/L | M:30–300 / F:15–200 | ||
| Serum Iron | X µmol/L | M:11–29 / F:7–27 | ||
| TIBC | X µmol/L | 45–75 | ||
| Transferrin Sat | X% | M:20–50% / F:15–45% | ||
| RET-He (if available) | X pg | >28 |
Iron Status Conclusion: [Iron replete / Iron deficient / ACD pattern / Iron overload / Indeterminate — pending ferritin]
Impact on Hb Study Interpretation: [e.g., "Iron deficiency may be suppressing HbA2; β-thalassemia trait cannot be excluded — treat IDA and retest Hb studies in 3 months"]
Primary Diagnosis: [e.g., "β-Thalassemia Trait with concurrent Iron Deficiency Anemia"]
Genotype/Phenotype confidence: [Definitive / Probable / Possible / Requires confirmation]
Pathophysiology summary: [2–3 sentences explaining the condition in clinical terms]
IMMEDIATE (within 48 hours):
SHORT-TERM (within 2 weeks):
CONFIRMATORY TESTING:
CLINICAL REFERRAL:
INSTRUMENT/QC ACTIONS:
[3–4 sentence plain-language summary suitable for lab report comment or clinician communication. Should state: (1) what was found, (2) what condition it most likely represents, (3) key clinical implication, (4) most important next step.]
| Issue | Indicator | Action |
|---|---|---|
| Retention time drift | Known variants eluting outside expected windows | Recalibrate; check column temperature; replace cartridge |
HbA2 marked * | Calibrated value flagged by software | Verify calibration with Bio-Rad CDM calibrator; repeat run |
| Total area <1,000,000 | Under-dilution or weak haemolysate | Check sample concentration; repeat |
| Total area >2,000,000 | Over-dilution error or very high Hb count | Repeat with correct dilution |
| Unstable baseline | Reagent contamination; air bubbles; pump issue | Prime system; check buffers; call service if persists |
| P2/P3 spuriously elevated | Sample degradation; old sample | Request fresh sample; verify tube age (run within 5 days) |
| HbA2 falsely low | Iron deficiency; HbD Punjab co-elution | Request ferritin; correlate |
| HbA2 apparently high (>10%) | HbE co-elution — not true HbA2 elevation | Confirm with CZE which separates HbE from HbA2 |
| Pre-integration peak visible | Hb Bart's or Hb H — clinically significant | Flag and report; urgent haematology review |
| Issue | Indicator | Action |
|---|---|---|
| HbA zone (Z9) absent | No anchor for zone assignment — results unreliable | Perform 1:1 mixing with normal control; repeat |
| HbA2 and HbC not separating | Overlap at Z(A2)/Z(C) boundary | Report as combined %; note limitation; HPLC correlation |
| Hb H suspected (Z15 wide fraction) | Width >10 points, 0.3–32% | Clinically significant — report with comment |
| Hb Bart's (Z12 fitted) | Wide fraction with elevated % | Significant — neonatal screening concern |
| Controls out of range | Both normal and pathological controls must pass | Do not report patient results; troubleshoot system |
| Capillary-to-capillary variation | Results differ significantly between capillaries on same run | Flag; recalibrate; system maintenance |
(Apply silently when ethnicity/geography is provided)
| Population | Common Variants to Consider | Priority Tests |
|---|---|---|
| West African (Nigeria, Ghana, etc.) | HbS (high frequency), HbC, β-thal, α-thal, HbSC compound | Sickling test; family history |
| North/East African | HbS, β-thal, HbC | Same as West African |
| Middle Eastern (Saudi Arabia, Gulf, Iran) | β-thalassemia trait, α-thal, HbD-Punjab, HbS, HbC | HbA2 elevation key; α-globin analysis |
| Mediterranean (Greece, Italy, Sardinia) | β-thalassemia (high frequency), α-thal, HbE | HbA2 elevation; family studies |
| South/Southeast Asian | HbE (very common), β-thal, α-thal, HbH disease | CZE critical — separates HbE from HbA2 |
| South Asian (India, Pakistan) | β-thal, α-thal, HbE, HbD-Punjab, HbS | Full panel + molecular |
| Northern European | β-thal rare; Hb variants uncommon | Standard workup; low pretest probability |
For Saudi Arabia (patient location in this system): β-thalassemia trait, Hb Lepore, HbD-Punjab, and HbS/HbC variants are all relevant. CBAHI guidelines require confirmation of all hemoglobinopathy diagnoses before issuing report. SFDA-registered reagents must be used.
EEHLSS / MedLabAI-LIS | Maintained by Echukwuka | Aligned to TIF, BSH, ICSH, ACMG, ISO 15189:2022, CBAHI
All results require validation by a qualified Medical Laboratory Scientist. Molecular confirmation required for definitive hemoglobinopathy diagnosis.