Artificial tethering of LC3 or p62 to organelles is not sufficient to trigger autophagy.
Friedemann LoosWei XieValentina SicaJosé Manuel Bravo-San PedroSylvie SouquèreGérard PierronSylvie LachkarAllan SauvatAdriana PetrazzuoloAna Joaquina JimenezFranck PerezMaria Chiara MaiuriOliver KeppGuido KroemerPublished in: Cell death & disease (2019)
The retention using selective hooks (RUSH) system allows to retain a target protein fused to green fluorescent protein (GFP) and a streptavidin-binding peptide (SBP) due to the interaction with a molar excess of streptavidin molecules ("hooks") targeted to selected subcellular compartments. Supplementation of biotin competitively disrupts the interaction between the SBP moiety and streptavidin, liberating the chimeric target protein from its hooks, while addition of avidin causes the removal of biotin from the system and reestablishes the interaction. Based on this principle, we engineered two chimeric proteins involved in autophagy, namely microtubule-associated proteins 1A/1B light chain 3B (MAP1LC3B, best known as LC3) and sequestosome-1 (SQSTM1, best known as p62) to move them as SBP-GFP-LC3 and p62-SBP-GFP at will between the cytosol and two different organelles, the endoplasmic reticulum (ER) and the Golgi apparatus. Although both proteins were functional in thus far that SBP-GFP-LC3 and p62-SBP-GFP could recruit their endogenous binding partners, p62 and LC3, respectively, their enforced relocation to the ER or Golgi failed to induce organelle-specific autophagy. Hence, artificial tethering of LC3 or p62 to the surface of the ER and the Golgi is not sufficient to trigger autophagy.
Keyphrases
- endoplasmic reticulum
- simultaneous determination
- cell death
- endoplasmic reticulum stress
- signaling pathway
- mass spectrometry
- oxidative stress
- liquid chromatography
- binding protein
- cell therapy
- solid phase extraction
- estrogen receptor
- stem cells
- tandem mass spectrometry
- quantum dots
- high resolution mass spectrometry
- breast cancer cells
- hiv infected
- dna binding
- hepatitis c virus
- gas chromatography