Pam3Cys promotes MSC proliferation, inhibits in vitro “wound healing,” and does not affect the MSC's ability to inhibit T-cell response. MSCs were plated in MSC medium and starved with 2% serum-containing media for 24 hours following 10% FCS-containing media with Pam3Cys. MSC proliferation was measured after 48 hours by ³H thymidine incorporation (Ai) and by cell count (Aii). Time response (Aiii) of an experiment similar to that in panel Aii, where MSCs were treated with medium alone (dashed line), 1 μg/mL Pam3Cys (dotted line), or 10 μg/mL Pam3Cys (solid line) were counted every 24 hours for 3 days. For migration assay, a round 5-mm diameter space was made in confluent MSC cultures and DMEM containing 10% FCS without (Bi,iii) or with (Bii,iv) 20 μg/mL Pam3Cys was added. Five days later, cells were fixed and stained. The diameters of the circles were measured and quantified in panel Bv. Original magnifications: × 10 (Biii-iv); × 6.3 (Bi-ii). The results represent the means ± SD of a total of 5 “wounds” in duplicate wells. For the immunosuppression assay, MSCs were incubated for 48 hours with 1 μg/mL Pam3Cys (□), 10 μg/mL Pam3Cys (yellow bars), 20 μg/mL Pam3Cys (⊡), or without Pam3Cys (▪), washed, and added to a T-cell line activated by its cognate antigen in different ratios. After 72 hours, cells were pulsed with 0.037 MBq (1 μCi) ³H thymidine and measured for ³H thymidine incorporation (C). The results represent the means ± SD of triplicate wells. *P < .05, Pam3Cys treatment versus medium alone, by 2-tailed Welch t test.