| Literature DB >> 32356544 |
Shama Sograte-Idrissi1, Thomas Schlichthaerle2, Carlos J Duque-Afonso3, Mihai Alevra4, Sebastian Strauss2, Tobias Moser3, Ralf Jungmann2, Silvio O Rizzoli5, Felipe Opazo6.
Abstract
A standard procedure to study cellular elements is via immunostaining followed by optical imaging. This methodology typically requires target-specific primary antibodies (1.Abs), which are revealed by secondary antibodies (2.Abs). Unfortunately, the antibody bivalency, polyclonality, and large size can result in a series of artifacts. Alternatively, small, monovalent probes, such as single-domain antibodies (nanobodies) have been suggested to minimize these limitations. The discovery and validation of nanobodies against specific targets are challenging, thus only a minimal amount of them are currently available. Here, we used STED, DNA-PAINT, and light-sheet microscopy, to demonstrate that secondary nanobodies (1) increase localization accuracy compared to 2.Abs; (2) allow direct pre-mixing with 1.Abs before staining, reducing experimental time, and enabling the use of multiple 1.Abs from the same species; (3) penetrate thick tissues more efficiently; and (4) avoid probe-induced clustering of target molecules observed with conventional 2.Abs in living or poorly fixed samples. Altogether, we show how secondary nanobodies are a valuable alternative to 2.Abs.Mesh:
Substances:
Year: 2020 PMID: 32356544 DOI: 10.1039/d0nr00227e
Source DB: PubMed Journal: Nanoscale ISSN: 2040-3364 Impact factor: 7.790