Control cells were treated for identical times with (middle lane)

Control cells were treated for identical times with (middle lane) 20 nM scrambled oligonucleotide. (bottom lane) beta actin antibody blots. 2b. Comparisons of the ratio of RPS2/actin from densitometry scans of the Western blots in fig. 2a. 2c. RT-PCR assays showing the relative level of RPS2 expression in (P) PC-3ML; (L) LNCaP; (IR)

pBABE-IBC-10a-c-myc; and (C) CPTX-1532 cells (at 90% confluent) which were (□) untreated or treated with (╪) scrambled oligonucleotide, and (░) 2 and (■) 4 ug/ml DNAZYM-1P for 8 hr. Shows that the DNAZYM-1P knocks out RPS2 mRNA expression in all 4 cell lines. (×) NPTX-1532 express low levels of RPS2 mRNA (value set at 1). RT-PCR vales selleck products were normalized relative to 18S RNA, and then the fold expression calculated relative to values for untreated NPTX-1532 cells which were set at 1. Results averaged from 3 experiments +/-1 S.D. Immunoflourescent labeling studies with RPS2 antibodies (i.e. P1 antibodies) revealed that RPS2 was over expressed in nuclear and cytoplasmic regions of untreated PC-3ML and CPTX-1532 cells (fig. 3). Figure 3 showed that following exposure of these cells to DNAZYM-1P (4 ug/ml) for 0 and 4 hr, the cells expressed an abundance of RPS2 (fig. 3). However, following extended treatments of 24 hr, the majority of the cells were negative

for RPS2. Control experiments showed that PC-3ML cells exposed to the scrambled DNAZYM oligonucleotide Vadimezan in vitro expressed RPS2 after 0, 4 and 24 hr. In comparison, NPTX-1532 cells which did not express RPS2, were unaffected by DNAZYM-1P for 0, 4 and 24 hr (fig. 3). IBC-10a parent cells also did not express RPS2 or respond to DNAZYM-1P treatment (data not shown). Figure 3 Immunolabeling of PC-3ML, CPTX-1532 and NPTX-1532 cells with RPS2 antibodies following treatment with 4 ug/ml DNAZYM-1P or scrambled oligonucleotide for 0, 4 and 24 hr. Cells were labeled with RPS2 P1 antibody (1:200 dil.) and Alexoflour secondary antibodies counterstained with DAPI. Cells were at ~70% confluence at the time treatment was AZD5582 purchase initiated.

Growth assays measured by the MTS assay [8] further ADAMTS5 showed that 4 and 6 ug/ml DNAZYM-1P blocked growth of 3 different malignant prostate cancer lines which over expressed RPS2, including PC-3ML (P:Z1, P:Z2), CPTX-1532 (C:Z1) and LNCaP (L:Z1) cells. In comparison, the scrambled oligonucleotide (P:scr) and lipofectamine (P:lip) alone did not block growth of PC-3ML cells. DNAZYM-1P treatment of NPTX-1532 (N:Z2) cells did not block cell proliferation (fig. 4a). Apoptosis Assays using Annexin V antibody labeling and flow cytometry showed that 4 & 6 ug/ml DNAZYM-1P induced increased amounts of apoptosis in PC-3ML cells after 8–24 hr (i.e. 5% to 28%) (fig. 4b, ■, ◆), but failed to induce significant amounts of apoptosis in NPTX-1532 cells after 0, 8, 24, 48 and 72 hr treatment (i.e. < 1.2%)(fig. 4c, ■, ◆).

AChR signal

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Control cells were treated for identical times with (middle lane)