PMC

All data were quantified in 2-Mb intervals. The top line shows summed EST data documenting the “transcriptional intensity” for each chromosomal interval (data from ). The bottom three lines show the summed frequency of integration site sequences in each interval. The numbers of ESTs (top) or integration sites (bottom three) are shown on the y-axis.

The human chromosomes are shown numbered. HIV integration sites from all datasets in Table 1 are shown as blue “lollipops”; MLV integration sites are shown in lavender; and ASLV integration sites are shown in green. Transcriptional activity is shown by the red shading on each of the chromosomes (derived from quantification of nonnormalized EST libraries, see text). Centromeres, which are mostly unsequenced, are shown as grey rectangles.

Human chromosome numbers are indicated at the bottom of the figure. The number of integration events detected in each chromosome was divided by the number expected from the matched random control. The line at one indicates the bar height expected if the observed number of integration events matched the expected number. Higher bars indicate favored integration, lower bars, disfavored integration. Most of the cell types studied were from human females; too little data were available for the Y chromosome for meaningful analysis.

Genes hosting integration events by the HIV vector were analyzed for their expression levels in transcriptional profiling data from IMR90, PBMC, and SupT1 cells. For each gene hosting an integration event, the expression values from the three cell types were then ranked lowest (red), medium (orange), and highest (yellow). The values were summed and displayed separately for each set of integration sites: (A) IMR90 sites, (B) PBMC sites, and (C) SupT1 sites. In each case there was a significant trend for the cell type hosting the integration events to show the highest expression values relative to the other two (p < 0.05 for all comparisons).

Genes or intergenic regions were normalized to a common length and then divided into ten intervals to allow comparison. The number of integration sites in each interval was divided by the number of matched random control sites and the value plotted. A value of one indicates no difference between the experimental sites and the random controls. Viruses and cell types studied are as marked above each graph. The direction of transcription within each gene is from left to right. Note that our normalization method de-emphasizes favored MLV integration events just upstream of gene 5′ ends (outside transcription units), as reported by . We carried out an analysis specially designed to identify this effect and confirmed that the regions just upstream of gene 5′ ends are favored for MLV integration when reanalyzed with the matched random control data (unpublished data).

Expression levels were assayed using Affymetrix HU-95Av2 or HU-133A microarrays and scored by the average difference value as defined in the Affymetrix Microarray Suite 4.1 software package. All the genes assayed by the chip were divided into eight “bins” according to their relative level of expression (the leftmost bin in each panel is lowest expression levels and the rightmost the highest). Genes that hosted integration events were then distributed into the same bins, summed, and expressed as a percent of the total. The y-axis indicates the percent of all genes in the indicated bin. P values were determined using the Chi-square test for trends by comparison to a null hypothesis of no bias due to expression level. All average difference values were ranked prior to analysis, and the analysis was carried out on the ranked data. This was done to avoid possible complications due to differential normalization or other data processing differences arising during work up of the microarrays.

The viral vectors and cell types studied are indicated by color. A value of one indicates no bias, less than one indicates disfavored integration, and more than one indicates favored integration. The x-axis (from plus or minus 1 kb to 50 kb) indicates distance from the edge of a CpG island in either direction along the genome. The statistical analysis specifically removed the favorable effects of being in a gene and being in a region containing expressed genes to highlight the effects of CpG islands alone. When effects of gene density and activity are left in, HIV integration goes from disfavored at short distances (less than 1 kb) to favored at longer distances (more than 10 kb). This is because at longer distances the association with genes is significant—many CpG islands are within 10 kb of a gene, and genes are favored targets for HIV integration. To carry out this analysis, the numbers of experimentally determined and matched control sites were fitted according to whether they were near a CpG island, whether they were in genes, and the level of the expression density variable. Each variable contributes a “multiplier” for the ratio of the number of experimental to control sites. The multiplier for “near CpG island” is shown (, p. 9–12).