Construction of PGRP-S^-/- mice. (A) Genomic organization of PGRP-S^+/+ and PGRP-S^-/- loci with 3 PGRP-S exons, genomic clones, targeting vector, and replacement of exon 1 with NEO cassette in PGRP-S^-/- mice. Relevant restriction sites, primers, and screening probes are also shown. (B) Genotypes of PGRP-S^-/-, PGRP-S^+/+, and PGRP-S^+/- mice determined by typing of genomic DNA by PCR using either PGRP-specific or NEO cassette–specific sense primer and intron-specific (S1) antisense primer. DNA from homozygous PGRP-S^-/- mice yielded only 320-bp NEO PCR fragment and no PGRP fragment, demonstrating the replacement of PGRP-S exon 1 with NEO cassette in both chromosomes. DNA from wild-type PGRP-S^+/+ mice yielded only 283-bp PGRP PCR fragment and no NEO fragment, whereas DNA from heterozygous PGRP-S^+/- mice yielded both PGRP and NEO PCR fragments. (C) Phenotypes of PGRP-S^-/- and PGRP-S^+/+ mice determined by Western blot: lysates of 2 × 10⁶ bone marrow cells/lane were separated by SDS-PAGE, and PGRP-S protein was detected by anti–PGRP-S antibodies on Western blots in lysates from PGRP-S^+/+ but not from PGRP-S^-/- mice.