Protein lysates were processed for immunoblots as described (Rutkowski et al, 2006 (link)). Primary antibodies include: CHOP (Santa Cruz sc-7351 RRID:AB_627411 for flow cytometry or Proteintech 15204-1-AP RRID:AB_2292610 for western blot), PARP (Cell Signaling Technology 9542 RRID:AB_2160739), ATF4 (Cell Signaling Technology 11815 RRID:AB_2616025), PeIF2α (Thermo 44-728G), total eIF2α (Cell Signaling Technology 9722 RRID:AB_2230924), and Calnexin (loading control; Enzo ADI-SPA-865 RRID:AB_10618434). Nanoluciferase activity was assessed using the Nano-Glo In-Gel Detection kit (Promega, USA) following the manufacturer’s protocol. qRT-PCR, including primer validation by standard curve and melt curve analysis, was also as described (Rutkowski et al, 2006 (link)). Briefly, RNA was isolated using Trizol (Thermofisher, USA) following the manufacturer’s protocol, and RNA concentrations were evaluated using the Qubit RNA Broad Range kit (Invitrogen, USA). 400 ng of RNA was used for reverse transcription using PrimeScript RT Master Mix (Takara, USA). PCR reactions were performed using TB Green Premix Ex Taq (Takara, USA). Gene expression was normalized against the average of two loading controls (Btf3 and Ppia).
Nano glo in gel detection kit
Manufactured by Promega
Sourced in United States
The Nano-Glo In-Gel Detection kit is a laboratory equipment product that enables the detection of luminescent proteins within polyacrylamide gels. The kit provides the necessary reagents to perform bioluminescent detection of target proteins after gel electrophoresis.
Automatically generated - may contain errors
Lab products found in correlation
Trizol, by Thermo Fisher Scientific (4 mentions)
Qubit broad range rna kit, by Thermo Fisher Scientific (2 mentions)
Primescript rt master mix, by Takara Bio (2 mentions)
Tb green premix ex taq, by Takara Bio (2 mentions)
Total eif2α, by Cell Signaling Technology (1 mentions)
P eif2α, by Thermo Fisher Scientific (1 mentions)
2 protocols using nano glo in gel detection kit
1
Immunoblot and qRT-PCR Protocol
2
Western Blot and qRT-PCR Protocol for Protein and Gene Expression Analysis
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Protein lysates were processed for immunoblots as described [24 (link)]. Primary antibodies include: CHOP (Santa Cruz sc-7351 for flow cytometry or Proteintech 15204–1-AP for western blot), PARP (Cell Signaling Technology 9542), and Calnexin (loading control; Enzo ADI-SPA-865). Nanoluciferase activity was assessed using the Nano-Glo In-Gel Detection kit (Promega, USA) following the manufacturer’s protocol. qRT-PCR, including primer validation by standard curve and melt curve analysis, was also as described [24 (link)]. Briefly, RNA was isolated using Trizol (Thermofisher, USA) following the manufacturer’s protocol, and RNA concentrations were evaluated using the Qubit RNA Broad Range kit (Invitrogen, USA). 400 ng of RNA was used for reverse transcription using PrimeScript RT Master Mix (Takara, USA). PCR reactions were performed using TB Green Premix Ex Taq (Takara, USA). Gene expression was normalized against the average of two loading controls (Btf3 and Ppia).
qRT-PCR Primers:
Btf3 forward: CCAGTTACAAGAAAGGCTGCT reverse: CTTCAACAGCTTGTCCGCT
Ppia forward: AGCACTGGAGAGAAAGGATT reverse: ATTATGGCGTGTAAAGTCACCA
FLuL exon1–2 forward: TTGAAGATGAGCGGGTGGCA reverse: CTTTCAGGTGTGGTGGTGTA
FLuL exon 2-nLuc forward: GTGTTCCAGAAGGAAGTGCA reverse: CTTTGGATCGGAGTTACGGA
FLuL exon 3–4 forward: GGAAGCCTGGTATGAGGAT reverse: CCACTCTGTTTCCGTTTCCT
qRT-PCR Primers:
Btf3 forward: CCAGTTACAAGAAAGGCTGCT reverse: CTTCAACAGCTTGTCCGCT
Ppia forward: AGCACTGGAGAGAAAGGATT reverse: ATTATGGCGTGTAAAGTCACCA
FLuL exon1–2 forward: TTGAAGATGAGCGGGTGGCA reverse: CTTTCAGGTGTGGTGGTGTA
FLuL exon 2-nLuc forward: GTGTTCCAGAAGGAAGTGCA reverse: CTTTGGATCGGAGTTACGGA
FLuL exon 3–4 forward: GGAAGCCTGGTATGAGGAT reverse: CCACTCTGTTTCCGTTTCCT
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