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Co precipitation assays All of the following measures had been carried

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 Co precipitation assays All of the following measures had been carried Empty Co precipitation assays All of the following measures had been carried

Сообщение  kai123 Пт Окт 17, 2014 11:18 am

The results clearly demonstrated the immunoprecipitated com plex containing JIP1 also contained JIP3 and kinesin one. This consequence may perhaps imply the physiological sig nificance of your association between JIP3 and JIP1. JIP3 enhances the association among JIP1 and kinesin 1 in Neuro2a cells To check whether or not JIP3 JIP1 binding is important to the asso ciation among JIP1 ATP-competitive JAK 阻害剤 and kinesin 1, we investigated the ef fect of JIP3 knockdown. Neuro2a cells stably expressing RFP tagged JIP1 had been transiently transfected with expression vectors for JIP3 shRNA or non silencing shRNA. Immunoprecipitation of RFP JIP1 followed by western blotting using anti KHC antibody uncovered the binding of RFP JIP1 and kinesin 1 was severely lowered by JIP3 knockdown.<br><br> We also examined no matter if the JIP3 knockdown altered the neurite tip localization of RFP JIP1. Differentiated RFP JIP1 Neuro2a cells were transiently transfected with shRNA vectors containing a GFP expression cassette to assist determine the transfected cells. The localization of RFP JIP1 towards the neurite tip of GFP labeled cells was signifi cantly diminished in shJIP3 LDE225 価格 transfected cells compared with NS transfected cells. The neurite tip localization of GFP was not observed in both the management cells or even the JIP3 knockdown cells. The kinesin one binding and neurite tip localization of RFP JIP1 diminished by JIP3 knockdown have been nearly recovered by the TAP JIP3 WT expression with out recovering the endogenous JIP3 level. These outcomes indicate that JIP3 is crucial for that association concerning JIP1 and kinesin one in Neuro2a cells.<br><br> LY2157299 臨床試験 Molecular basis for JIP1 JIP3 kinesin one ternary complex formation As shown in Figure 2C, the ectopic expression of JIP3 in HEK293T cells enhanced the association between JIP1 and kinesin one. To confirm the result of JIP3 depends on the binding of JIP3 to your JIP1 PTB domain, we per formed co precipitation assays working with the JIP1 F687V mu tant, which showed negligible binding to JIP3. Even though the expression of GFP JIP3 enhanced the binding of TAP tagged JIP1 WT to kinesin one, the impact of JIP3 expres sion was negated by the JIP1 F687V mutation. Concomitant binding of GFP JIP3 was sig nificantly decreased from the F687V mutation.<br><br> Nonetheless, inside the absence of JIP3, the weak kinesin 1 binding exercise on the JIP1 F687V mu tant was comparable with that of JIP1 WT, indicating the F687V mutation isn't going to influence the basal bind ing capacity of JIP1 to kinesin 1. This basal kinesin one binding capacity was dependent to the C terminal sequence of JIP1. These outcomes indicate that JIP1 JIP3 complicated formation through F687 significantly increases the kinesin 1 binding capacity of JIP1, compared with JIP1 alone. We confirmed that roughly equal amounts of V5 KHC and V5 KLC have been present within the JIP1 pull down fraction. This suggests that V5 KHC and V5 KLC type the kinesin 1 holoenzyme in HEK293T cells and bind to JIP1. We then sought to clarify why the JIP1 JIP3 complex showed such greater kinesin one binding exercise. Because each JIP1 and JIP3 can bind to kinesin one, we examined irrespective of whether the binding of JIP3 to kinesin one is crucial to the secure binding in the JIP1 JIP3 complicated to kinesin one.

kai123

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