Logo Allmyblog
Logo Allmyblog
Lien de l'article    

MAKINGMACHINE

dfgb
Contacter l'auteur de ce blog

CATEGORIES
- dfgbd

5 DERNIERS ARTICLES
- Altogether the three Republicans won 57 percent
- Your security system should have alarms
- Just another source of cost and replacement labor
- The built-in microprocessor system can control the luminous intensity
- LED let you use either normal white light
Sommaire

CALENDRIER
LunMarMerJeuVenSamDim
01
02030405060708
09101112131415
16171819202122
23242526272829
3031
<< Octobre >>

BLOGS FAVORIS
Ajouter makingmachine à vos favoris

LIENS FAVORIS
- LED Filament Bulb
 GAL4-cJun luciferase reporter assays Alerter l'administrateur Recommander à un ami Lien de l'article 

GAL4-cJun luciferase reporter assays in cerebellar granule neurons
Cerebellar granule neurons were transfected with a firefly luciferase reporter plasmid driven by five GAL4 elements in tandem, pGL3-G5E4Δ38 (12.5% of total DNA), pcDNA3-GAL4cJun plasmid encoding the transactivation domain of c-Jun (residues 5–105) fused to the DNA-binding domain of GAL4 (residues 1–147; 12.5% of total DNA), and pRL-CMV (12.5% of total DNA) expressing sea pansy luciferase as an internal standard against which signals were normalized24. CMV was selected for normalization because pcDNA3-GAL4cJun is also driven by CMV promoter. To activate the JNK pathway, either pEBG-ΔMEKK1 (10% of total DNA), a plasmid encoding MAPK-kinase kinase 1 (MEKK1) kinase domain (amino acids 1,174–1,493) was co-transfected, or cells were subjected to 4?h of WTS. Differentially targeted mCherry-OptoJNKi constructs or empty vector (mCherry-C1) were co-transfected as indicated. For WTS experiments, all OptoJNKi constructs were transfected at 40% of total DNA. For the specific case of ΔMEKK1-co-expression experiments, mCherry-3xNLS-OptoJNKi was transfected at 40% of total DNA but pilot titration evaluations indicated light-independent artefacts at high levels of the NES-targeted form; by transfecting at only 2% of total DNA, we avoided effects in dark conditions, as can be seen in the figures. We did not find a suitable percentage level for use of H2B-OptoJNKi in ΔMEKK1-transfected cells, suggesting a possible unexpected interaction between these two constructs, so we were unable to use H2B-OptoJNKi in this specific JNK-activation model, even though there was no evidence of dark effects of H2B-OptoJNKi in the WTS model. This emphasizes the need for careful titration of constructs and inclusions of appropriate controls in every model. But this is not unique to OptoJNKi as the risks of overexpression are well known, potentially affecting use of ΔMEKK1 and most other constructs. It should be noted that, in cerebellar neuron cultures as used here, the 10% level of ΔMEKK1 plasmid used had little impact on overall expression as judged by Renilla luciferase internal control signal, but it substantially increased the GAL4-cJun-driven firefly luciferase response. For the ΔMEKK1 plates, 2?h after transfection, wells were individually illuminated as indicated. Illumination was carried out using blue LEDs (peak 465–467?nm) with 500?Hz pulsed-width modulation to achieve 0.6?mW?cm?2 incident power on the well bottom (duty cycle modulation was set according to measured LED Tube China at 100% duty cycle using an Ex-Cite XR2100 power meter from Lumen Dynamics/LDGI, Mississauga, Ontario, Canada). The illumination was delivered in pulses of 1.5?s length or as indicated. Pulses were repeated with periodicity and for time windows as indicated in the figures. For ΔMEKK1 experiments, dual luciferase reporter assay was carried out on samples lysed 18–20?h after transfection. For the WTS plates, conditioned cell culture medium was replaced by minimal essential medium (cat# 11700) 20?h after transfection and wells were maintained in a cell culture incubator (Cytomat 2C, Thermo) for a further 4?h before lysis, under the illumination conditions described. Dual luciferase reagent (Promega) was used to assay firefly (reporter) and Renilla (internal standard) luciferase activities in samples lysed in passive-lysis buffer (Promega) according to the manufacturer’s instructions24.

  Aucun commentaire | Ecrire un nouveau commentaire Posté le 06-06-2017 à 08h37

 « Article précédant Retour à l'accueil du blog Article suivant »

 Articles dans la même catégorie
- Altogether the three Republicans won 57 percent

- Your security system should have alarms

- Just another source of cost and replacement labor

- The built-in microprocessor system can control the luminous intensity

- LED let you use either normal white light

- Light bulbs are often available in a variety of colors

- LED light bars have proven to be most effective

- They are mobile and easily relocated according to requirements


 Liste des commentaires Ecrire un nouveau commentaire


 Ajouter un commentaire
Titre
Commentaire
:) ;) :o :D :s :( :@ :clown: :$ :star: +o( ^|
8( :] (6) (h) :p 9| :'( (y) (n) :| 8-| :{
:?: :nrv: (l) (u) :o/ :pig: :hand: (h5) :yin: :nuc: :x ;D
Auteur
E-Mail (facultatif)
Blog (facultatif)
Se souvenir de mes informations
Recopier le code ci-contre :


SYNDICATION
 
Fil RSS 2.0
Ajouter à NetVibes
Ajouter à Google
Ajouter à Yahoo
Ajouter à Bloglines
Ajouter à Technorati
http://www.wikio.fr
 

Allzic en direct

Liens Commerciaux
L'information à Lyon
Retrouvez toute l'actu lyonnaise 24/24h 7/7j !


L'information à Annecy
Retrouvez toute l'actu d'Annecy 24/24h 7/7j !


L'information à Grenoble
Retrouvez toute l'actu de Grenoble 24/24h 7/7j !


Application Restaurant
Restaurateurs, demandez un devis pour votre application iPhone


Fete des Lumières
Fête des lumières : vente de luminaires, lampes, ampoules, etc.

Votre publicité ici ?
  Blog créé le 16-05-2017 à 08h36 | Mis à jour le 11-08-2017 à 03h24 | Note : Pas de note