CCK 8 analysis mean was firstly performed to analyze the influence of JNK and JAK STAT inhibitors on NHL cells proliferation. As shown in Figure 7A, both SP600125 and STATTIC could significantly decrease the proliferation rate of NHL cells. To further investigate whether ISL 1 was involved in the inhibition of tumor cells proliferation mediated by these inhibitors, Ly3 cells were treated with SP600125 or STATTIC to inhibit the phosphorylation of c Jun or STAT3. As shown in Figure 7B, C and, a distinct decreased e pression of ISL 1 was correlated to SP600125 or STATTIC induced inhibition of p c Jun or p STAT3. Additionally, the e pression change of c Myc was also consistent with the change pattern of ISL 1. These data indicate that the JNK and JAK STAT pathways regulate c Myc e pression and NHL cells proliferation, which may be partly through the regulation of ISL 1 e pression.

To e plore this further, luciferase assay was used to analyze the impact of SP600125 or STATTIC on the luciferase activity of c Myc luc. The inhibition of JNK and JAK STAT pathways significantly decreased c Myc luc activity, and the overe pression of ISL 1 could recover the effect mediated by the inhibitors of JNK and JAK STAT pathways. Whereas, the mutant constructs c Myc luc M1 e hibited much smaller e tent of luciferase activity changes. These results support that ISL 1 is involved in the JNK and JAK STAT regulation on c Myc e pression. We ne t assessed whether the e pression level of ISL 1 could influence the effects of p c Jun and p STAT3 on the proliferation rate of Ly3 cells.

As shown in Figure 7E, both p c Jun and p STAT3 inhibitors could significantly suppress the proliferation of Ly3 cells transfected with the control vectors, while, the growth inhibition mediated by p c Jun and p STAT3 inhibitors could be rescued in ISL 1 overe pressing cells, which further demonstrates the effect of ISL 1 on the proliferation of cells. Collectively, JNK and JAK STAT signaling inhibitors suppress NHL cells proliferation possibly through down regulating ISL 1 e pression. Therefore, ISL 1 may serve as a new target molecule for NHL treatment. p STAT3 p c Jun ISL 1 forms a transcriptional comple and binds directly to the ISL 1 promoter in NHL cells The above results have shown that p STAT3 and p c Jun could increase the e pression level of ISL 1 to promote the proliferation of NHL cells.

However, it is unknown how p STAT3 and p c Jun control ISL 1 e pression. Bio informatic analysis showed that the core transcriptional regulatory region of ISL 1 contains conserved p STAT3 and p c Jun binding sites. Luciferase assay with ISL 1 luc, a ISL 1 luciferase reporter construct containing the binding site of c Jun and STAT3, Batimastat was performed in Ly3 cells treated with IL 6 STATTIC or Anisomycin SP600125, respectively. As shown in Figure 8B, ISL 1 luc activity was increased in Anisomycin or IL 6 treated cells.