2c–f). To assess this further, the CD27+CD43+ quadrant was broken into two smaller regions comprising either CD27+CD43+lo–int cells or CD27+CD43+hi
cells (Fig. 2b,d,f). The more stringent the CD20+ gating, the fewer cells that were present in the CD27+CD43hi region (Fig. 2f). This was therefore named the ‘contamination region’, while the CD27+CD43lo–int region was entitled ‘putative B1 cells’ (Fig. 2c,f). We then postulated whether the cells in the contamination region were either T cells expressing CD43 or cell doublets. To examine this further, cells from the pure B1 cell region and the contamination region were analysed for CD3 expression and assessed for size using forward-scatter–pulse width (FSC-W) to indicate the proportion MG-132 cell line of doublet cells being measured (Fig. 3). Figure 3d,i shows the proportion of contaminating cells that ICG-001 price are CD19–CD3+ in both a relaxed and a stringent CD20 gating strategy, respectively. The median proportion of cells within the contamination gate under relaxed CD20 gating that were CD3+CD19– was 31·4% (IQR: 14·5–43·9%), compared to 22·2% (IQR: 17·1–39·7%) CD3+CD19– cells in the contamination gate
under stringent CD20 gating (n = 13). More importantly, the median proportion of CD3+CD19– cells present in the ‘putative B1 cell’ with relaxed CD20 gating was 0·6% (IQR: 0·2–1·3%); this was compared to only 0·2% (IQR: 0·0–0·4%) CD3+CD19– cells in the pure B1 cell region with stringent CD20 gating (Fig. 3b,g). These Fenbendazole data together indicate that not only is stringent CD20 gating required to help remove contaminants from the CD27+CD43+ B cell compartment but also that CD27+CD43lo–int putative B1 cell gating is required, as the CD27+CD43hi contamination compartment, even with stringent CD20 gating, showed a high percentage of CD3+CD19– cells. Doublet analysis showed a minor contribution to the proportion of
contaminated cells compared with single CD3+CD19– cells (Fig. 3e). This was raised slightly in the contamination gate using strict CD20 gating, but was postulated to be due to the reduced number of cells in this region (Fig. 3j). From this point forth all future experiments were carried out using the CD20+CD27+CD43lo–int phenotype as the definition of human putative B1 cells. Previous reports show that human B1 homologue cells appear to decline with age [12]. The CD20+CD27+CD43lo–int cell percentage within CD20+ and CD27+ B cells was 4·1% (3·3–5·6%) and 18·7% (8·6–23·1%) in the healthy controls [median (IQR)], respectively, with no significant difference between both sexes (P = 0·81) (data not shown). Within CD20+ B cells, we found a moderate negative correlation of the CD20+CD27+CD43lo–int cells proportion with age (r = −0·4, P = 0·02) (data not shown).