Genomic and real-time PCR transcriptional analysis of the KIR repertoire. (A) The size of the NK-cell compartment was analyzed by flow cytometry (% CD3−CD56+CD16+ cells) in exposed HIV-infected IDU (HIV, ▴) exposed HIV-uninfected IDU (EU, •), and unexposed control blood donors (C, □). (B) Real-time PCR analysis of altered KIR transcript patterns in HIV and EUs. KIR2DL4, KIR3DL2, KIR2DL3, and KIR3DL1 mRNA transcript levels are represented as relative copy numbers per 106GAPDH transcripts. KIR2DL3 transcript levels where examined according to the alternative KIR2DL3+KIR2DS2−KIR2DL2− or KIR2DL3+KIR2DS2+KIR2DL2+ genomic gene combinations (middle left) and also plotted according to the size of the phenotypically defined GL183+ NK-cell subset (middle right). A high percentage of GL183+ NK cells (> 50% of GL183+ NK cells within CD3−CD56+ NK cells) identified a specific subgroup of KIR2DL3+KIR2DS2−KIR2DL2− EU individuals who exhibit higher KIR2DL3 transcript levels in the absence of KIR2DS2/KIR2DL2 transcription (boxed area). Activating KIR3DS1/inhibitory KIR3DL1 transcript ratio is represented (bottom right). EUs with higher KIR3DS1/KIR3DL1 ratios as compared with C and HIV+ are boxed. Horizontal bars represent the median and the 25th and 75th percentiles.