2016
DOI: 10.3390/proteomes4040036
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Let There Be Light!

Abstract: The invention of the microscope has been fundamental for the understanding of tissue architecture and subcellular structures. With the advancement of higher magnification microscopes came the development of various molecular biology tools such as Förster resonance energy transfer (FRET) and in situ proximity ligation assay (in situ PLA) to monitor protein interactions. Microscopy has become a commonly used method for the investigation of molecular events within the cell, for the identification of key players i… Show more

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Cited by 17 publications
(19 citation statements)
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“…To investigate VAMP7-rhodopsin interactions in situ, we employed the established proximity ligation assay (PLA), modified for the analysis of vertebrate retinas, where it detects transient rhodopsin interaction with the ciliary targeting complex exclusively in the RIS (Wang and Deretic, 2015;Wang et al, 2017Wang et al, , 2012. Through the fluorescent signalwhich is only present when the PLA probes are <40 nm apart, a distance within the limits of protein-protein interactions (Raykova et al, 2016;Söderberg et al, 2006) we detected potential VAMP7-rhodopsin interaction sites along the entire Golgi/TGN-to-cilia pathway (Fig. 1E, red dots, arrows).…”
Section: Resultsmentioning
confidence: 99%
See 1 more Smart Citation
“…To investigate VAMP7-rhodopsin interactions in situ, we employed the established proximity ligation assay (PLA), modified for the analysis of vertebrate retinas, where it detects transient rhodopsin interaction with the ciliary targeting complex exclusively in the RIS (Wang and Deretic, 2015;Wang et al, 2017Wang et al, , 2012. Through the fluorescent signalwhich is only present when the PLA probes are <40 nm apart, a distance within the limits of protein-protein interactions (Raykova et al, 2016;Söderberg et al, 2006) we detected potential VAMP7-rhodopsin interaction sites along the entire Golgi/TGN-to-cilia pathway (Fig. 1E, red dots, arrows).…”
Section: Resultsmentioning
confidence: 99%
“…The PLA was performed using Duolink in situ Detection Reagents Red, containing specific secondary antibodies attached to oligonucleotides. Circular DNA is formed when oligonucleotides are less than <40 nm apart; it is amplified and hybridized to fluorescently labeled oligonucleotides that generate an output in a form of red fluorescent dots of ∼0.5 µm in size, which are visualized by microscopy (Raykova et al, 2016;Söderberg et al, 2006). Only previously validated antibodies were used for this assay.…”
Section: Confocal Microscopy Clem and Plamentioning
confidence: 99%
“…The method can be considered as an in situ mimic of an "immunoprecipitation assay". Proximity ligation assays can identify a protein-protein interaction/association with a distance of 10-30 nm that is in the upper range of that observed using FRET (5-20 nm) and this methodology can detect authentic endogenous proteins in situ that does not rely on transfected or artificially GFPtagged protein vectors [45]. We evaluated whether IFITM1/3 and HLA-B co-associate using this methodology using antibodies to HLA-B and Mab-MHK (that can bind to both IFITM1 and IFITM3 proteins; Supplementary Fig.…”
Section: Orthogonal Validation Of Ifitm1/3 Dependent Induction Of Hlamentioning
confidence: 99%
“…1E. To pinpoint the localization of GBF1 within the Golgi, we performed in situ proximity ligation assay (PLA), a molecular technique suitable for proteomic analysis, because a positive signal is possible only when the fluorescent PLA probes are <40 nm apart (Raykova et al, 2016;Söderberg et al, 2006). We employed PLA modified for studies of brain and retinal tissue (Blasic et al, 2012;Trifilieff et al, 2011;Wang and Deretic, 2015;Wang et al, 2012;Zulliger et al, 2015).…”
Section: Resultsmentioning
confidence: 99%