DNA origami demonstrate the unique stimulatory power of single pMHCs as T cell antigens

Hellmeier, Joschka; Platzer, René; Eklund, Alexandra S.; Schlichthaerle, Thomas; Karner, Andreas; Motsch, Viktoria; Schneider, Magdalena C.; Kurz, Elke; Bamieh, Victor; Brameshuber, Mario; Preiner, Johannes; Jungmann, Ralf; Stockinger, Hannes; Schütz, Gerhard J.; Huppa, Johannes B.; Sevcsik, Eva

doi:10.1073/pnas.2016857118

Cited by 81 publications

(90 citation statements)

References 56 publications

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“…For the quantitative comparison of different functionalization strategies, we employed a recently introduced platform 6 based on rectangular DNA origami tiles anchored to a fluid-phase supported lipid bilayer (SLB) via cholesterol-modified oligonucleotides 25 . DNA origami constructs were assembled from a 65x54 nm DNA origami tile 1 featuring a centrally located and elongated staple strand to create a target for quantitative functionalization with proteins (SI Fig.…”

Section: Resultsmentioning

confidence: 99%

“…S1). As protein we selected for this study a monovalent single-chain antibody fragment of the variable domain derived from the TCRβreactive monoclonal antibody H57-597 (H57-scFV) 26 , which was shown to induce T-cell activation when displayed on SLBs 6,27 . We further equipped the H57-scFV C-terminally with either a biotin ligase recognition sequence or an unpaired cysteine for the site-specific attachment to DNA origami structures, that would not interfere with TCR binding (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…Given that exact placement of proteins within DNA origami structures is a primary reason for their use in the first place, this obvious lack of experimental control diminishes the usefulness of tetravalent streptavidin in many biological and biophysical applications. In fact, we have previously observed that the presence of only 0.5% DNA origami structures carrying two H57-scFVs at a distance of 10 nm instead of a single H57-scFV dominates T-cell activation behavior 6 with obvious consequences for the kind of conclusions that can be drawn from such experiments.…”

Section: For Each Dose-response Curve Data Are From At Least Two Independent Experiments Involving T-cells Isolated From Two Different MImentioning

confidence: 99%

“…By using short oligonucleotides ("staples") to guide the folding of a long single stranded DNA scaffold, it is not only possible to program the shape of a DNA origami structure but also to arrange functional elements with nanometer resolution and precision 1 . Proteindecorated DNA origami structures have thus far been interfaced with cells as soluble agents 2,3 , attached to a solid substrate 4,5 or anchored to a fluid supported lipid bilayer (SLB) 6,7 ; biological questions addressed range from studying cellular signaling and adhesion processes [2][3][4][5][6]8,9 , to creating synthetic multienzyme cascades 10,11 to more and more elaborate robotic DNA machines 12 .…”

mentioning

confidence: 99%

“…While this may be acceptable for some applications, many mechanistic studies, e.g. those focusing on receptor-ligand interactions 2,3,6 , depend on the functionalization with not more than one protein at a specific site. We have recently circumvented this potential shortcoming of streptavidin by using divalent SAv (dSAv) 24 as a connector to strictly avoid double or triple occupancies at a single modification site 6 .…”

mentioning

confidence: 99%

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Strategies for the site-specific decoration of DNA origami nanostructures with functionally intact proteins

Hellmeier

Platzer

Muehlgrabner

et al. 2021

Preprint

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DNA origami structures provide flexible scaffolds for the organization of single biomolecules with nanometer precision. While they find increasing use for a variety of biological applications, the functionalization with proteins at defined stoichiometry, high yield, and under preservation of protein function remains challenging. In this study, we applied single molecule fluorescence microscopy in combination with a cell biological functional assay to systematically evaluate different strategies for the site-specific decoration of DNA origami structures, focusing on efficiency, stoichiometry and protein functionality. Using an activating ligand of the T-cell receptor (TCR) as protein of interest, we found that two commonly used methodologies underperformed with regard to stoichiometry and protein functionality. While strategies employing tetravalent wildtype streptavidin for coupling of a biotinylated TCR-ligand yielded mixed populations of DNA origami structures featuring up to 3 proteins, the use of divalent (dSAv) or DNA-conjugated monovalent streptavidin (mSAv) allowed for site-specific attachment of a single biotinylated TCR-ligand. The most straightforward decoration strategy, via covalent DNA conjugation, resulted in a 3-fold decrease in ligand potency, likely due to charge-mediated impairment of protein function. Replacing DNA with charge-neutral PNA in a ligand conjugate emerged as the coupling strategy with the best overall performance in our study, as it produced the highest yield with no multivalent DNA origami structures and fully retained protein functionality. With our study we aim to provide guidelines for the stoichiometrically defined, site-specific functionalization of DNA origami structures with proteins of choice serving a wide range of biological applications.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: For Each Dose-response Curve Data Are From At Least Two Independent Experiments Involving T-cells Isolated From Two Different MImentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Strategies for the site-specific decoration of DNA origami nanostructures with functionally intact proteins

Hellmeier

Platzer

Muehlgrabner

et al. 2021

Preprint

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Harnessing DNA Nanotechnology for Nongenetic Manipulation and Functionalization of Cell Surface Receptor

Nan,

Wang,

Nie

2024

DNA Nanotechnology for Cell Research

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Engineering DNA Nanostructures to Manipulate Immune Receptor Signaling and Immune Cell Fates

Tseng

Wang

Douglas

et al. 2021

Adv Healthcare Materials

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Immune cells sense, communicate, and logically integrate a multitude of environmental signals to make important cell-fate decisions and fulfill their effector functions. These processes are initiated and regulated by a diverse array of immune receptors and via their dynamic spatiotemporal organization upon ligand binding. Given the widespread relevance of the immune system to health and disease, there have been significant efforts toward understanding the biophysical principles governing immune receptor signaling and activation, as well as the development of biomaterials which exploit these principles for therapeutic immune engineering. Here, how advances in the field of DNA nanotechnology constitute a growing toolbox for further pursuit of these endeavors is discussed. Key cellular players involved in the induction of immunity against pathogens or diseased cells are first summarized. How the ability to design DNA nanostructures with custom shapes, dynamics, and with site-specific incorporation of diverse guests can be leveraged to manipulate the signaling pathways that regulate these processes is then presented. It is followed by highlighting emerging applications of DNA nanotechnology at the crossroads of immune engineering, such as in vitro reconstitution platforms, vaccines, and adjuvant delivery systems. Finally, outstanding questions that remain for further advancing immune-modulatory DNA nanodevices are outlined.

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DNA origami demonstrate the unique stimulatory power of single pMHCs as T cell antigens

Cited by 81 publications

References 56 publications

Strategies for the site-specific decoration of DNA origami nanostructures with functionally intact proteins

Strategies for the site-specific decoration of DNA origami nanostructures with functionally intact proteins

Harnessing DNA Nanotechnology for Nongenetic Manipulation and Functionalization of Cell Surface Receptor

Engineering DNA Nanostructures to Manipulate Immune Receptor Signaling and Immune Cell Fates

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