Whole blood (WB) samples (100 µl) from PNH patients were provided by the College of American Pathologists (CAP; Northfield, IL, USA) and UK NEQAS (London, UK) between May 2017 and August 2017. WB samples (100 µl) from 10 healthy donors (aged 58.4±11.1 years) were also collected. The samples were stored in BD Vacutainer™ blood collection tubes containing EDTA as an anti-coagulant (BD Biosciences, Franklin Lakes, NJ, USA) at 4°C and tested within a month. For certain experiments, PNH proficiency test samples were obtained from CAP and UK NEQAS. Alexa Fluor (A)488-conjugated FLAER was purchased from Cedarlane (Burlington, ON, Canada). Phycoerythrin (PE)-conjugated anti-CD157 (SY/11B5), Allophycocyanin (APC)-conjugated anti-CD24 (ALB9) and APC-A750-conjugated anti-CD64 (clone 22) were purchased from Beckman Coulter, Inc. (Brea, CA, USA). Peridinin chlorophyll protein complex (PerCP)-conjugated anti-CD14 (MfP9), PE-cyanine (Cy)7-conjugated anti-CD5 (L17F12), PE-Cy7-conjugated anti-CD19 (SJ25C1), V450-conjugated anti-CD15 (MMA), V500-C-conjugated anti-CD45 (2D1), PerCP-Cy5.5-conjugated anti-CD3 (SK7), APC-conjugated anti-CD4 (SK3), APC-H7-conjugated anti-CD8 (SK1), V450-conjugated anti-CD7 (M-T701), PE-conjugated anti-CD55 (IA10) and APC-conjugated anti-CD14 (MfP9) were purchased from BD Biosciences. All the antibodies were titrated to optimize the cocktail performance. The present study was reviewed by the Research Determination Office of Kaiser Permanente (Oakland, CA, USA) and determined not to be human research due to the use of secondary de-identified samples; therefore, the requirements of informed patient consent and ethical approval were waived.

The 8-color antibody cocktail for PNH detection was prepared according to the configuration listed in Table I. A total of 1×10⁶ cells in the EDTA-whole blood samples were transferred to 12×75 mm Falcon tubes and stained with the 8-color cocktail antibody cocktail for 15 min at room temperature in dark. The whole blood was then lysed with 2 ml BD FACS™ Lysing Solution (BD Biosciences) for 10 min at room temperature. After washing the cells twice with phosphate-buffered saline (PBS; Beckman Coulter, Inc.) and resuspending in 0.5 ml 0.5% paraformaldehyde as fixation buffer (Polysciences, Inc., Warrington, PA, USA), data were acquired on a BD FACSCanto™ II flow cytometer with standard configuration (BD Biosciences). A total of 100,000 events in the monocyte and granulocyte cell gates were acquired. BD FACSDiva™ v.6.1.3 software under standard 8-color configuration (BD Biosciences) was used for acquisition and analysis. For compensation, a BD™ Comp Beads kit was used to create cocktail-specific compensation matrices on whole blood from the healthy donors utilizing batch-matched single color reagents following the manufacturer's instructions. For a 4-color control experiment, PE-CD55 (10 µl), APC-CD14 (5 µl), FLAER-A488 (10 µl) and V500-C-CD45 (5 µl) were used to stain four normal whole blood samples (100 µl each). For certain experiments, whole blood was stained with PerCP-Cy5.5-CD3, APC-CD4, V450-CD7 and APC-H7-CD8.

The percentage of PNH clones [FLAER⁻/CD157⁻ on CD64⁺ granulocytes (Grans)] was determined using the 8-color cocktail listed in Table I. Three PNH samples were spiked in 100 µl normal whole blood to obtain a final concentration of PNH clones of 0.5–2%. They were then serial diluted at 1:1 (v:v) using normal whole blood as diluent up to 0.005–0.01% expected PNH percentage (Table II). Unspiked normal whole blood was used as a negative control. Following preparation of the serial dilutions, the samples were stained with the 8-color cocktail following the staining procedure described above. A total of 100,000 events in the monocyte and granulocyte gates were acquired for each sample. CD15⁺ Grans FLAER⁻/CD157⁻ PNH clones were identified on CD157/FLAER dot plots.

Data acquisition was performed with FCS Express 5 (De Novo Software, Glendale, CA, USA) and BD FACSDiva™ v.6.1.3 using gating strategy on dot plots, after which appropriate subsets were identified.

To assess the correlation of CD15⁺ Grans FLAER⁻/CD157⁻ PNH clones between expected and actual percentages, a linear regression analysis was performed. All statistical calculations were performed with Excel 2016 (Microsoft Corporation, Redmond, WA, USA) and Prism 7 (GraphPad Software, Inc., La Jolla, CA, USA). R²>0.95 and P-value <0.0001 were considered to indicate significant correlation.

In the present study, a whole blood sample from a healthy donor was stained with a 4-color cocktail containing FLAER-A488, PE-CD55, APC-CD14 and V500-C-CD45. From this, a minor CD55⁻ granulocyte population was observed (Fig. 1). However, this population was FLAER⁺, suggesting that it was not representative of PNH clones, which have been determined to be FLAER⁻ (26). Three other normal samples exhibited the same FLAER⁻/CD55⁺ population of granulocytes (data not shown).

To increase the sensitivity of multicolor flow cytometry, the present study aimed to remove non-specific binding and artifacts. A normal blood sample was stained with a multicolor cocktail targeting T cell markers (CD3, CD4, CD8 and CD7). A number of artifacts were identified in the granulocytes and monocytes regions on CD3/SSC, CD4/SSC, CD8/SSC and CD7/SSC plots (Fig. 2, indicated in red). Other lymphocyte markers including CD25 exhibited the same artifacts (data not shown). Some of those artifacts were doublets and could be eliminated by doublet discrimination (data not shown). However, some artifacts remained following gating out of all doublets as observed on the CD19+CD5/SSC plot in Fig. 3 (green arrow).

To determine whether the 8-color PNH panel was able to identify PNH clones, blood samples spiked with PNH clones were stained with an 8-color PNH cocktail (Table I). The forward scatter width and height (FSC-W and -H) were used to gate the singlets population. Monocytes and granulocytes were gated together and non-specific binding events were removed by gating the negative population on the ‘dump’ channel (CD5 and CD19; Fig. 3). A number of artifacts were identified on the right side of the granulocyte and monocyte region on the CD5+CD19/side scatter (SSC) plot, and those events were eliminated by gating the negative populations of monocytes and granulocytes, resulting in reduced background (Fig. 3). The monocyte antigen CD64 and granulocyte antigen CD15 further separated monocytes and granulocytes, respectively. The PNH clones exhibited negativity for FLAER and GPI-linked antigens (CD157, CD24 and CD14; Fig. 3). The CD5⁺CD19⁺ population was present together with CD15⁺ Grans, CD64⁺ Mono and affected FLAER⁻/CD157⁻ quadrant as indicated in Fig. 4 (top panel; green population). There were FLAER⁻/CD157⁻ differences that ranged from 0.014 to 1.28% when excluding or including the CD5⁺CD19⁺ populations (Fig. 4, lower panel). By contrast, normal whole blood stained with the same 8-color PNH cocktail did not exhibit any events on the lower left quadrant of FLAER/CD157, FLAER/CD24 and FLAER/CD14 plots (Fig. 5, top panel). The samples of 10 normal donors were stained with this 8-color PNH cocktail and exhibited an average of 0.002773±0.001743% PNH clones (FLAER⁻/CD157⁻) in the CD15⁺ Gran population and 0.000764±0.002415% in the CD64⁺ monocyte population, respectively (Fig. 5, lower panel). These results suggest that the 8-color assay has high specificity.

The percentage of PNH clones in three PNH samples were determined using the 8-color panel. The PNH samples were then spiked into normal whole blood to attain a final PNH concentration of 0.5–2%, and serial dilutions were performed. The first tube of sample 1 exhibited 2.2% PNH clones (FLAER⁻/CD157⁻), and was subsequently diluted in 50% increments until it reached 0.01% (Fig. 6). The normal whole blood control did not exhibit a PNH population on the left lower quadrant of the FLAER/CD157 plot (Fig. 6). The actual number of FLAER⁻/CD157⁻ events in sample 1 was 10/69,216 CD15⁺ Grans at the lower limit of detection (LOD) of 0.014% (Fig. 6 and Table III). The number of FLAER⁻/CD157⁻ events in samples 2 and 3 at the corresponding LODs were 10/73,469 CD15⁺ Grans and 8/77,229 CD15⁺ Grans, respectively (Table III); samples 1–3 exhibited an LOD for FLAER⁻/CD157⁻CD15⁺ Grans of 0.01% (Table III) and 0.05% for CD64⁺ Mono (data not shown) on the 8-color flow assay. The expected PNH clone percentage was significantly correlated with the actual value, R² value of 0.9839 and p value less than 0.0001 on a linear curve (Fig. 7), suggesting that the 8-color PNH flow assay had high sensitivity, detecting a PNH clone population as low as 0.01% in CD15⁺ Grans.

The percentages of PNH clones in the CAP and UK-NEQAS samples were determined using the 8-color panel. The percentage of FLAER⁻/CD157⁻ Grans in the CAP sample was 8.79%, which matched the CAP FLAER/CD157 granulocytes specification (4.70–10.00%; Fig. 8). The percentage of FLAER⁻/CD157⁻ Mono in the CAP sample was 7.89%, which matched the CAP FLAER⁻/CD157⁻ monocytes specification (7.39–10.13%; Fig. 8). Furthermore, the percentage of two UK-NEQAS samples identified by the 8-color assay matched the UK-NEQAS specifications (Fig. 8), suggesting that the 8-color flow assay had high accuracy for PNH clone identification.