Abstract
The advancement of new immunotherapies for the treatment of cancers, infections, immune- mediated inflammatory diseases, and autoimmune diseases necessitates the co-development of appropriate probes to detect and monitor the distribution and infiltration of distinct immune cell populations. Considering the key role of CD4+ T cells in regulating immunological processes, we have developed a set of novel single-domain antibodies (nanobodies, Nbs) that specifically recognize the human CD4 co-receptor in its native state on various CD4+ cells. Following detailed characterization of binding properties, epitope mapping, and site-directed functionalization, we selected biologically inert Nbs that do not affect T cell proliferation or cytokine expression in vitro. We used fluorescently labeled Nbs to track the presence and location of CD4+ cells in a xenograft model, demonstrating a high signal-to-background ratio by in vivo optical imaging. In summary, this study reports for the first time the generation and application of human CD4-specific Nbs for the detection and in vivo imaging of CD4+ cells in a preclinical animal model. We anticipate that the Nbs presented in this study will be versatile probes, e.g. in immunoPET imaging for patient stratification and for monitoring individual immune responses during personalized immunotherapy.
Introduction
In precision medicine, diagnostic classification of the disease-associated immune status should guide the selection of appropriate therapies (1–3). A comprehensive analysis of a patient’s specific immune cell composition, activation state, and infiltration of affected tissue has been shown to be highly informative for patient stratification. When administering immunotherapeutics, this enables the prediction of responders and non-responders, the monitoring of therapeutic efficacy, and the detection of serious adverse events even before symptoms occur (4–8). CD4+ T cells are a key determinant of the immune status due to their essential role in orchestrating immune responses in T cell-mediated delayed hypersensitivity reactions in autoimmune diseases, inflammation, cancer, and chronic viral infections (9–16). Accordingly, detailed monitoring of the dynamic distribution of CD4+ T cells is highly relevant for companion diagnostics. Currently, the presence, activation and differentiation state of CD4+ T cells can be assessed and monitored in the peripheral blood of patients revealing only the systemic immune cell status. More comprehensive diagnostic measures from biopsies of tumors or of immune-mediated inflammatory diseases (IMIDs) are enabled by a range of methods including intra-cytoplasmic flow cytometry analysis (IC-FACS), cytometry by time of flight (CyTOF), immunohistochemistry and ex vivo cytokine assays or RT-PCR analysis (17–21). However, because of the heterogeneity of cancers and the CD4+ T cell infiltrate in IMIDs, biopsies provide only spatially and temporally restricted information about the CD4+ T cell infiltrate, which does often not reflect the holistic immune profile. Considering the emerging role of infiltrating lymphocytes and the impact of CD4+ T cells on the outcome of immunotherapies novel approaches are needed to assess CD4+ T cells throughout the entire tumor, all metastases, or the affected tissue of IMIDs (22, 23). In this context, non-invasive imaging approaches offer a significant benefit compared to the current diagnostic standard. To date, radiolabeled antibodies have been applied to image CD4+ T cells in preclinical models (13, 24–26). Due to the recycling effect mediated by the neonatal Fc receptor, full-length antibodies have a long serum half-life (∼ 1–3 weeks), which requires long clearance times (several days) before high-contrast images can be acquired (27). Additionally, effector function via the Fc region was shown to induce depletion or functional changes in CD4+ cells including the induction of proliferation or cytokine release (28–30). Notably, also higher dosages of recombinant antibody fragments like the Fab fragment or a Cys-diabody derived from the monoclonal anti-CD4 antibody GK1.5 were recently shown to cause a decrease in CD4 expression in vivo and inhibit proliferation and IFN-γ production in vitro (29–31). These studies highlight the importance of carefully investigating CD4+ T cell-specific immunoprobes for their epitopes, binding properties, and functional effects.
During the last decade antibody fragments derived from heavy-chain-only antibodies of camelids (32), referred to as VHHs or nanobodies (Nbs) (32), emerge as novel probes for molecular imaging (reviewed in (33)). Nbs are characterized by a small size, antibody-like affinities and specificities, low off-target accumulation, high stability and good solubility (reviewed in (34, 35)). Their unique properties and ease of genetic and/or chemical functionalization offer significant advantages over conventional antibodies and recombinant fragments thereof. Additionally, Nbs were described as weakly immunogenic in humans due to their high homology to the human type 3 VH domain (VH3) (36). In combination with highly sensitive and/or quantitative whole-body molecular imaging techniques such as optical imaging or radionuclide-based techniques (e.g. positron emission tomography (PET)), Nbs have been shown to bind their targets within several minutes of systemic application (37). Due to their great potential as highly specific imaging probes, numerous Nbs targeting immune- or tumor-specific cellular targets are currently in preclinical development and even in clinical trials (33, 38, 39).
Here, we generated a set of human CD4-specific Nbs, examined their binding properties on recombinant and cellular CD4, and determined their epitopes with sub-domain resolution. A series of immunological analyses were performed to evaluate their impact on T cell proliferation and activation, as well as cytokine production in isolated human peripheral blood mononuclear cells (PBMCs) and whole blood. For non-invasive in vivo optical imaging, we converted the most promising candidates into CD4 immunoprobes by site-directed fluorescent labeling and investigated their ability to visualize human CD4-positive tissue in a murine xenograft model.
Results
Generation of high-affinity CD4 nanobodies
To generate Nbs directed against human CD4 (hCD4), we immunized an alpaca (Vicugna pacos) with the recombinant extracellular portion of hCD4 following an 87-day immunization protocol. Subsequently, we generated a Nb phagemid library comprising ∼4 × 107 clones that represent the full repertoire of variable heavy chains of heavy-chain antibodies (VHHs or Nbs) of the animal. We performed phage display using either passively adsorbed purified hCD4 or CHO and HEK293 cells stably expressing full-length human CD4 (CHO-hCD4, HEK293-hCD4 cell lines). Following two cycles of phage display for each condition, we analyzed a total of 612 individual clones by whole-cell phage ELISA and identified 78 positive binders. Sequence analysis revealed 13 unique Nbs representing five different B cell lineages according to their complementarity determining regions (CDR) 3 (Figure 1 A). One representative Nb of each lineage, termed CD4-Nb1 – CD4-Nb5, was expressed in bacteria (E.coli) and isolated with high purity using immobilized metal ion affinity chromatography (IMAC) followed by size exclusion chromatography (SEC) (Figure 1 B). To test whether selected Nbs are capable of binding to full-length hCD4 localized at the plasma membrane of mammalian cells, we performed live-cell staining of CHO-hCD4 cells (Figure 1 C, Supplementary Fig. 1). Executed at 4°C, images showed a prominent staining of the plasma membrane, whereas at 37°C the fluorescent signal was mainly localized throughout the cell body, presumably a consequence of endocytotic uptake of receptor-bound Nbs. CHO wt cells were not stained by any of the five CD4-Nbs at both temperatures (data not shown). CD4-Nb1 and CD4-Nb3, both identified by whole-cell panning, displayed strong staining of CHO-hCD4 cells. Of the Nbs derived from panning with recombinant hCD4, CD4-Nb2 also showed strong cellular staining, whereas staining with CD4-Nb4 revealed weak signals. CD4-Nb5 showed no staining under these conditions and was consequently excluded from further analyses (Figure 1 C). To quantitatively assess binding affinities, we performed biolayer interferometry (BLI) measuring serial dilutions of Nbs on the biotinylated extracellular domain of hCD4 immobilized at the sensor tip. For CD4-Nb1 and CD4-Nb2, determined KD values ∼5 and ∼7 nM, respectively, while CD4-Nb3 and CD4-Nb4 displayed lower affinities of 75 nM and 135 nM, respectively (Figure 1 D, Table 1, Supplementary Fig. 2 A). In addition, we determined corresponding EC50 values with full-length plasma membrane-located hCD4 on HEK293-hCD4 cells by flow cytometry. In accordance with cellular staining and biochemically determined affinities these values revealed a strong functional binding for CD4-Nb1 and CD4-Nb2 with EC50 values in the subnanomolar range (∼0.7 nM), whereas CD4-Nb3 and CD4-Nb4 displayed substantially lower cellular affinities (Figure 1 E, Table 1, Supplementary Fig. 2 B). In summary, we generated four CD4-Nbs that bind isolated as well as cell-resident hCD4. While CD4-Nb3 and CD4-Nb4 appeared less affine, CD4-Nb1 and CD4-Nb2 displayed high affinities in the low nanomolar range.
Domain mapping
Next, we applied chemo-enzymatic coupling using sortase A for site-directed functionalization of CD4-Nbs (40, 41). We thereby linked peptides conjugated to a single fluorophore to the C- terminus of CD4-Nbs yielding a defined labeling ratio of 1:1 (42). Live-cell immunofluorescence imaging showed that all sortase-coupled CD4-Nbs retained their capability of binding to cell- resident hCD4 of CHO-hCD4 cells (Supplementary Fig. 3 A). To localize the binding sites of the selected CD4-Nbs, we generated domain-deletion mutants of hCD4. Expression and correct surface localization of these mutants in CHO cells was confirmed by staining with antibody RPA-T4 binding to domain 1 of CD4. For mutants lacking domain 1, we introduced an N-terminal BC2 tag (43) to allow for live-cell surface detection with a fluorescently labeled bivBC2-Nb (42) (Supplementary Fig. 3 B). Transiently expressed domain-deletion mutants were then tested for binding of CF568-labeled CD4-Nbs by live-cell immunofluorescence imaging, including a non-specific fluorescently labeled GFP-binding Nb (GFP-Nb) as negative control. Based on these results, we allocated binding of CD4-Nb1 and CD4-Nb3 to domain 1, whereas CD4-Nb2 and CD4-Nb4 bind to domain 3 and/or 4 of hCD4 (Figure 2 A, Supplementary Fig. 3 C).
To further examine combinatorial binding of the different CD4-Nbs, we performed an epitope binning analysis by BLI. Recombinant full-length hCD4 was immobilized at the sensor tip and combinations of CD4-Nbs were allowed to bind consecutively (Supplementary Fig. 4). Unsurprisingly, CD4-Nbs binding to different domains, displayed combinatorial binding. Interestingly, a simultaneous binding was also detected for the combination of CD4-Nb1 and CD4-Nb3, suggesting that both CD4-Nbs bind to different epitopes within domain 1. In contrast, we did not observe simultaneous binding for CD4-Nb2 and CD4-Nb4, which might be due to close-by or overlapping epitopes at domain 3/4 for the latter Nb pair.
For a more precise epitope analysis, we conducted a hydrogen-deuterium-exchange (HDX) mass spectrometry analysis of hCD4 bound to CD4-Nb1, CD4-Nb2 or CD4-Nb3 (Figure 2 B- E). Due to its low affinity, CD4-Nb4 was not considered for HDX-MS analysis (data not shown). In accordance with our previous findings, binding of CD4-Nb1 and CD4-Nb3 protected sequences of domain 1 from HDX, whereas CD4-Nb2 protected sequences of domain 3 and 4 of hCD4 (Figure 2 B). The results obtained for binding of CD4-Nb1 (Figure 2 C) are similar to those obtained for CD4-Nb3 (Figure 2 D) in that binding of either Nb reduced hydrogen exchange at amino acid residues (aa) from aa T17 to N73, albeit with a different extent of protection at individual sequence segments. For CD4-Nb1 the greatest protection from HDX was observed for the sequence ranging from aa K35 – L44 corresponding to β strand C’ and C’’ of the immunoglobulin fold of domain 1 and residues aa K46 – K75, comprising β strands D and E. In contrast, binding of CD4-Nb3 confers only a minor reduction in HDX within the latter sequence, but additionally protects sequence aa C84 – E91, which correspond to β strands G and F and their intermediate loop. For CD4-Nb2 we found protection of sequences aa W214 – F229 (β strands C and Ć) and aa K239 – L259 (β strands C’’-E), and to a minor extend sequence aa R293 - L296 as part of β strands A of domain 4 (Figure 2 E). In summary, our HDX-MS analysis revealed that all three tested Nbs bind three dimensional epitopes within different parts of hCD4. It further provides an explanation how CD4-Nb1 and CD4-Nb3 can bind simultaneously to domain 1 of hCD4, and confirms that the epitope of CD4-Nb2 is mainly located at domain 3.
Binding of CD4-Nbs to human PBMCs
Having demonstrated that all selected Nbs bind to recombinant and exogenously overexpressed cellular hCD4, we next examined their capability and specificity of binding to physiologically relevant levels of CD4+ T cells within PBMC samples. We co-stained human PBMCs from three donors with CD4-Nbs1-4 coupled to CF568 (100 nM for high-affine CD4- Nb1 and CD4-Nb2; 1000 nM for low-affine CD4-Nb3 and CD4-Nb4) in combination with an anti-CD3 antibody and analyzed the percentage of double-positive cells (CD3+CD4+) by flow cytometry (Figure 3 A, Supplementary Fig. 5). Compared to staining with an anti-CD4 antibody used as positive control, all CD4-Nbs stained a similar percentage of CD4+ T cells for all tested donors, while the non-specific GFP-Nb yielded a negligible percentage of double- positive cells even at the highest concentration (1000 nM) (Figure 3 B, Table 2).
Impact of CD4-Nbs on activation, proliferation and cytokine release of CD4+ T and immune cells
Towards the envisioned application as clinical imaging tracer, we next assessed basic issues associated with CD4-Nbs, regarding their influence on the activation, proliferation and cytokine release of CD4+ T cells. First, to exclude adverse effects of bacterial endotoxins present in the CD4-Nbs1-4 preparations, we attempted to remove endotoxins by depletion chromatography to yield FDA-acceptable endotoxin levels of <0.25 EU per mg. While this was achieved for CD4-Nb1, CD4-Nb4 and the non-specific GFP-Nb, we failed to lower protein-associated endotoxins to acceptable levels for CD4-Nb2 and CD4-Nb3 even after repeated depletion chromatography. Consequently, we continued these experimental studies only with CD4-Nb1, CD4-Nb4 and GFP-Nb as control. In brief, carboxyfluorescein succinimidyl ester (CFSE)- labeled human PBMCs from three pre-selected healthy donors were pre-treated with CD4-Nbs or a control Nb at concentrations between 0.05 µM – 5 µM for 1 h at 37°C, mimicking the expected approximate concentration and serum retention time during clinical in vivo imaging application. Cells were then washed to remove Nbs and stimulated with an antigenic (cognate MHCII peptides) or a non-antigenic stimulus (phytohaemagglutinin, PHA-L) and analyzed after 4, 6 and 8 days by flow cytometry with the gating strategy shown in Supplementary Fig. 6 A. According to the highly similar CFSE intensity profiles observed, the total number of cell divisions was not affected by the different Nb treatments (exemplarily shown for one of three donors on day 6, Supplementary Fig. 6 A). For samples of the same donor and time point, no substantial differences in the percentage of proliferated cells were observed between mock incubation and individual Nb treatments.
For both stimuli, the average percentage of proliferated cells increased over time in all donors tested, with no clear differences between conditions (Figure 4 A). As quantitative measure of T cell activation, we also determined the cell surface induction of a very early activation marker (CD69) and of the IL-2 receptor α chain (CD25) on CD4+ T cells (Figure 4 B). Among samples of the same donor and stimulation, we found highly similar activation profiles for all Nb treatments. While the percentage of CD4+CD25+ cells steadily increased over time for MHCII peptide stimulation, for PHA-stimulated condition the percentage of positive cells was similarly high at all times of analysis. Importantly, regardless of the differences between donors, the individual Nb treatments from the same donor did not result in significant differences in the percentage of CD4+CD25+ or CD4+CD69+ cells for either stimulation at any point in the analysis.
Next, we analyzed cytokine expression of CD4+ T cells by intracellular cytokine staining after restimulation with cognate MHCII peptides. The corresponding gating strategy is shown in Supplementary Fig. 6 B. Samples of the same donor treated with different Nbs had highly similar percentages of cytokine (TNF, IFN-γ or IL-2) or activation marker (CD154)-positive cells without stimulation and upon stimulation with MHCII peptides (Figure 4 C). Overall, exposure to CD4-Nbs did not affect proliferation, activation or cytokine production of CD4+ T cells. In addition, we analyzed potential effects of CD4-Nbs on the release of cytokines from full-blood samples of three further donors. Upon stimulation with lipopolysaccharide (LPS) or PHA-L, we determined the serum concentrations with a panel of pro- and anti-inflammatory cytokines (Supplementary Table S2). Although there was significant inter-donor variation for some cytokines, Nb treatment did not result in significant differences in either stimulated or unstimulated samples (Supplementary Fig. 7).
In vivo optical imaging of CD4-Nbs
For optical in vivo imaging, we labeled CD4-Nbs with the fluorophore Cy5.5 (CD4-Nb-Cy5.5) by sortase-mediated attachment of an azide group followed by click-chemistry addition of DBCO-Cy5.5. First, we tested potential cross-reactivity of the four Cy5.5-labeled CD4-Nbs to murine CD4+ lymphocytes. Notably, flow cytometric analysis showed that none of the selected CD4-Nbs was able to bind murine CD4+ cells, suggesting exclusive binding to human CD4. Moreover, low-affine binding CD4-Nb4 bound neither mouse nor human CD4+ cells at the concentration used here (0.75 µg/ml, ∼49 nM) (Supplementary Fig. 8). Consequently, we focused on CD4-Nb1 as the most promising candidate and CD4-Nb4 as a candidate with a high off-target rate, both of which we further analyzed for their in vivo target specificity and dynamic distribution using a murine xenograft model.
To establish human CD4+ expressing tumors, NSG mice were inoculated subcutaneously with CD4+ T cell leukemia HPB-ALL cells (44). After 2 – 3 weeks, mice bearing HPB-ALL xenografts were injected with 5 µg of CD4-Nb1-Cy5.5, CD4-Nb4-Cy5.5, or a control Nb (GFP-Nb-Cy5.5) and optically imaged in intervals over the course of 24 h (Figure 5 A, Supplementary Fig. 9 A). The Cy5.5 signal intensity (SI) of the control Nb peaked within 10 – 20 minutes and rapidly declined thereafter to approximately the half and a quarter of maximum level at 2 h and 24 h, respectively (Figure 5 B, Supplementary Fig. 9 B). While the SI of the low-affinity CD4-Nb4- Cy5.5 did not exceed the SI of the control Nb at any time (Supplementary Fig. 9 B), CD4- Nb1-Cy5.5 reached its maximum SI within the HPB-ALL xenograft of ∼1.8-fold above the control Nb, at 30 min and slowly declined to ∼90% and ∼80% of maximum after 2 and 4 hours, respectively (Figure 5 B). Based on the differences in the SI between CD4-Nb1-Cy5.5 and GFP-Nb-Cy5.5, we observed the optimal target accumulation and specificity between 60 and 120 min post injection (Figure 5 B). After 24 h, mice were euthanized, and the presence of fluorophore-labeled CD4 Nbs within the explanted tumors was analyzed by optical imaging (OI) (Figure 5 C, Supplementary Fig. 9 C). Compared to control, tumors from mice injected with CD4-Nb1-Cy5.5 had ∼4-fold higher Cy5.5 SI, indicating a good signal-to-background ratio for this Nb-derived fluorescently labeled immunoprobe. To confirm CD4-specific targeting of CD4-Nb1 within the xenograft, we performed ex vivo immunofluorescence of HPB-ALL tumors at 2 h and 24 h post injection (Supplementary Fig. 10). At the early time point, when the in vivo OI signal peaked, CD4-Nb1 was widely distributed throughout the whole tumor whereas no Cy5.5 signal was detected in the GFP-Nb-injected mice (Supplementary Fig. 10 A, B). Semiquantitative analysis at the single-cell level revealed intense CD4-Nb1 binding at the surface of HBP-ALL cells that correlated with the CD4 antibody signal and internalization of CD4-Nb1 in some cells (Supplementary Fig. 10 C). Upon administration of unrelated GFP- Nb, no Nb binding was observed (Supplementary Fig. 10 D). 24 h post injection we observed regions of strongly internalized CD4-Nb1 (Supplementary Fig. 10 E, G), but also regions showing a low residual CD4-Nb1 uptake (Supplementary Fig. 10 E, H).
Although the HBP-ALL xenograft model used for in vivo imaging does not reflect the natural distribution of CD4+ T cells in an organism, the provided data strongly indicates that high- affinity binding CD4-Nb1 is suitable for visualizing CD4+ cells in vivo by non-invasive imaging.
Discussion
Prognosis and therapeutic susceptibility to immunotherapies are critically influenced by the presence and activity of various subsets of immunological cells, including members of the innate and adaptive immunity. The role of immune cells in influencing the outcome of e.g. cancer therapy, is generally recognized (45, 46). Among the latter, T cells acquire functional and effector phenotypes whose activities have direct pro- or anti-inflammatory consequences (47). In this context, CD4+ T helper 1 (Th1) cells for example promote anti-tumoral responses by secretion of proinflammatory cytokines such as IL-2, TNF, and IFN-γ, which promotes cytotoxic CD8+ T cell (CTL) priming and cytotoxicity (48). CD4, a co-receptor of the T cell receptor (TCR) complex, is predominantly expressed by T helper and regulatory T cells and plays an important role in the recognition of major histocompatibility complex class II (MHCII) molecules expressed on antigen-presenting cells (49). In addition, minor levels of CD4 are also expressed on monocytes, macrophages, NK cells and dendritic cells. Upon interaction of CD4 with MHCII, CD4+ T cells become activated, recruiting other immune cells and assist the transformation of B cells to antibody-producing plasma cells and thereby guiding pro- and anti- inflammatory responses. With respect to cancer, the presence of infiltrating CD4+ Th1 cells in tumors correlates with a favorable prognosis in terms of overall survival and disease-free survival in many malignancies (48). However, cancer cells can also recruit regulatory CD4+ T cells (Tregs), which suppress many of the anti-tumor activities and have been reported to negatively regulate CTLs and activated CD4+ T cells by exploiting the peripheral tolerance mechanism via checkpoint engagement (50–53).
Given this important role of CD4+ T cells, their detailed monitoring is proving to be highly relevant for the concomitant diagnosis not only of cancer (reviewed in (12)), but also of other diseases, including viral infections (13–16) and autoimmune diseases (9–11). Several mouse studies and early clinical trials already indicated the value of non-invasive imaging of CD4+ cells in rheumatoid arthritis (25), colitis (26), allogenic stem cell transplantation (54), organ transplant rejection (55), acquired immunodeficiency disease (13), and in the context of cancer immunotherapies (56), using radiolabeled full-length antibodies or fragments thereof.
However, biological activity, particularly CD4+ T cell depletion, and long-term systemic retention of full-length antibodies limit their development into clinically applied immunoprobes (25, 29, 57, 58).
In this study, we developed novel Nbs as immunoprobes for the visualization and monitoring of human CD4+ cells in various biomedical research applications, focusing on non-invasive in vivo imaging. To identify binders that recognize the cellular exposed CD4 receptor, we generated a Nb phage display library from an alpaca immunized with the extracellular portion of recombinant human CD4 and employed two screening strategies. First, we performed phage display against adsorbed recombinant CD4 and second, we used whole cells stably expressing human CD4. Interestingly, both strategies proved successful, as demonstrated by the selection of two Nbs that efficiently bind cell-resident CD4 from each panning strategy.
To determine key information regarding their stabilities, affinities, and recognized epitopes on human CD4, these Nbs were subjected to in-depth biochemical characterization. Using epitope binning, cellular imaging, and HDX-MS, we were able to elucidate in detail the detected domains, as well as the three-dimensional epitopes addressed by the individual Nbs, and thus identified two candidates, CD4-Nb1 and CD4-Nb3, that can simultaneously bind different segments within domain 1, while CD4-Nb2 has been shown to bind domain 3 of CD4. Notably, such detailed information is not available for most Nbs currently developed for in vivo imaging (59–65). However, for CD4-specific Nbs this knowledge is all the more important because epitope-specific targeting of CD4+ T cell functions have far-reaching implications. This is true especially for cancer treatment, as CD4+ cells have opposing effects on tumor growth and response to immunotherapies, crucially depending on the CD4 effector cell differentiation and tumor entity (66, 67). In this context it was shown that domain 1 of CD4 mediates transient interaction of the CD4 receptor and the MHCII complex (68–70), while T cell activation is abrogated when TCR and CD4 colocalization is blocked via domain 3 (71).
To further elucidate a possible impact on immunomodulation, we analyzed the effect of CD4- Nb1 and CD4-Nb4 targeting two different domains on CD4+ T cell proliferation and cytokine expression. Notably, here we used Nb concentrations as they are proposed to be applied for molecular imaging purposes in patients. In summary, none of the Nbs seems to affect the behavior of endogenous CD4+ T cells in vitro or induce increased cytokine levels in whole blood samples. From these data it can be concluded that these Nbs are mostly biologically inert and thus might be beneficial compared to full-length antibodies (29) or other antibody fragments such as the anti-CD4 cys-diabody, which was recently reported to inhibit proliferation of CD4+ cells and IFN-γ production in vitro (31).
Finally, we provide first data on the performance of our CD4-Nbs for in vivo imaging applications. Facing the challenge that the selected CD4 Nbs bind exclusively to human CD4 but not to the homolog in mice, we used a murine xenograft model in which we implemented a CD4+ T leukemia tumor model based on human-derived HBP-ALL cells. For optical imaging, we performed a site-directed labeling approach employing C-terminal sortagging to conjugate an azide group, which can be universally used to attach a multitude of detectable moieties by straightforward DBCO-mediated click chemistry (59). By optical in vivo imaging, we monitored the specific enrichment of the high-affine CD4-Nb1 but not of the low-affine CD4-Nb4 on HBP- ALL-derived xenografts. A twofold signal-to-background ratio within 120 min after application and a rapid decrease in Nb-derived fluorescence intensities after 24 h suggest that the CD4- Nb1 is well suited to identify CD4+ cells in vivo.
Undoubtedly, these first promising results still need to be confirmed in a more physiologically relevant in vivo model. Therefore, we are considering a humanized CD4 mouse model to further investigate CD4-Nb1-mediated visualization of CD4+ T cells under physiologically relevant conditions. In parallel, we have begun to convert our CD4 Nbs into corresponding radiolabeled immunoPET imaging probes using the combination of sortagging and subsequent click-mediated, site-directed attachment of the detectable portion, as described in this study. We propose that PET imaging with radiolabeled CD4-Nbs will meet the clinical needs of tracking CD4+ T cells non-invasively with high resolution and appropriate sensitivity.
As mentioned previously, epitope-specific targeting of CD4+ T cell functions by Nbs might also be beneficial for novel therapeutic approaches (72). Consequently, beyond application as a diagnostic agent, CD4 Nbs offer various therapeutic opportunities. We now have started to investigate the impact of targeted binding of mono- or biparatopic CD4 Nbs to modulate protein interactions and downstream signaling of CD4, thus exploiting the potential of Nbs as functional modulators.
In summary, this study demonstrates for the first time the generation and detailed characterization of Nbs specific for human CD4 and their comprehensive experimental evaluation in vitro and in vivo. In particular, CD4-Nb1 is a promising candidate for the non- invasive, whole-body study of CD4+ T cells in mice, as well as in humans. In the next step, we will convert the CD4-Nb1 into an immunoPET tracer to quantify and monitor the infiltration of CD4+ T cells in different tumor types using a humanized CD4 mouse model.
Data availability
The data that support the findings of this study are available from the corresponding author upon reasonable request.
Authorship Contributions
B.T., M.K., D.S., B.P. and U.R. designed the study; S.N., A.S. immunized the animal; P.D.K., S.H., Y.P. performed Nb selection; P.D.K, B.T., M.W., T.R.W., A.M. performed biochemical characterization and functionalization of Nbs; M.G., A.Z. performed MS analysis; A.Z. and M.G. performed HDX-MS experiments; J.R., C.G., M.J., N.S.M. analyzed the Nb effects on T cell proliferation and cytokine expression; S.P., and D.S. performed in vivo imaging; M.S. performed staining of xenograft cryosections; B.T., J.R., C.G., M.K., B.P., D.S. and U.R. drafted the manuscript; M.K., B.P. and U.R. supervised the study.
Competing financial interests
D.S., M.K., B.P., B.T., P.D. K., U.R. are named as inventors on a patent application claiming the use of the described nanobodies for diagnosis and therapeutics filed by the Natural and Medical Sciences Institute and the Werner Siemens Imaging Center. The other authors declare no competing interest.
Materials and Methods
Nanobody library generation
Alpaca immunization and Nb library construction were carried out as described previously (73, 74). Animal immunization has been approved by the government of Upper Bavaria (Permit number: 55.2-1-54-2532.0-80-14). In brief, an alpaca (Vicugna pacos) was immunized with the purified extracellular domains of human CD4 (aa26-390) recombinantly produced in HEK293 cells (antibodies-online GmbH, Germany). After initial priming with 1 mg, the animal received six boost injections with 0.5 mg hCD4 each, every second week. 87 days after initial immunization, ∼100 ml of blood were collected and lymphocytes were isolated by Ficoll gradient centrifugation using Lymphocyte Separation Medium (PAA Laboratories GmbH). Total RNA was extracted using TRIzol (Life Technologies) and mRNA was transcribed into cDNA using the First-Strand cDNA Synthesis Kit (GE Healthcare). The Nb repertoire was isolated in 3 subsequent PCR reactions using the following primer combinations (1) CALL001 and CALL002, (2) forward primer set FR1-1, FR1-2, FR1-3, FR1-4 and reverse primer CALL002, and (3) forward primer FR1-ext1 and FR1-ext2 and reverse primer set FR4-1, FR4- 2, FR4-3, FR4-4, FR4-5 and FR4-6 introducing SfiI and NotI restriction sites. The Nb library was subcloned into the SfiI/ NotI sites of the pHEN4 phagemid vector (75).
Nb screening
For the selection of CD4-specific Nbs two consecutive phage enrichment rounds were performed, both with immobilized recombinant antigen and CHO-hCD4 cells. E.coli TG1 cells comprising the hCD4-Nb-library in pHEN4 were infected with the M13K07 helper phage to generate Nb-presenting phages. For each round 1 × 1011 phages of the hCD4-Nb-library were applied on immunotubes coated with hCD4 (10 µg/ml). In each selection round extensive blocking of antigen and phages was performed with 5% milk or BSA in PBS-T and with increasing panning rounds PBS-T washing stringency was increased. Bound phages were eluted in 100 mM tri-ethylamine, TEA (pH10.0), followed by immediate neutralization with 1 M Tris/HCl pH7.4. For cell-based panning, 2 × 106 CHO-hCD4 or HEK293-hCD4 were non-enzymatically detached using dissociation buffer (Gibco) and suspended in 5% fetal bovine serum (FBS) in PBS. Antigen expressing cells were incubated with 1 × 1011 phages under constant mixing at 4°C for 3 h. Cells were washed 3 × with 5% FBS in PBS. Cell lines were alternated between panning rounds. Phages were eluted with 75 mM citric acid buffer at pH2.3 for 5 min. To deplete non-CD4-specific phages, eluted phages were incubated 3 × with 1 × 107 wt cells. Exponentially growing E.coli TG1 cells were infected with eluted phages from both panning strategies and spread on selection plates for following panning rounds. Antigen- specific enrichment for each round was monitored by counting colony forming unit (CFUs).
Whole-cell phage ELISA
Polystyrene Costar 96-well cell culture plates (Corning) were coated with poly-L-lysine (Sigma Aldrich) and washed once with H2O. CHO-wt and CHO-hCD4 were plated at 2 × 104 cells per well in 100 µl and grown to confluency overnight. Next day, 70 µl of phage supernatant was added to culture medium of each cell type and incubated at 4°C for 3 h. Cells were washed 5 × with 5% FBS in PBS. M13-HRP-labeled antibody (Progen) was added at a conc. 0.5 ng/ml for 1 h, washed 3 × with 5% FBS in PBS. Onestep ultra TMB 32048 ELISA substrate (Thermo Fisher Scientific) was added and incubated until color change was visible and the reaction was stopped by addition of 100 µl of 1M H2SO4. Detection occurred at 450 nm at a Pherastar plate reader and phage ELISA-positive clones were defined by a 2-fold signal above wt control cells.
Expression constructs
The cDNA of human CD4 (UniProtKB - P01730) was amplified from hCD4-mOrange plasmid DNA (hCD4-mOrange was a gift from Sergi Padilla Parra; addgene plasmid #110192; http://n2t.net/addgene:110192; RRID:Addgene_110192) by PCR using forward primer hCD4 fwd and reverse primer hCD4 rev and introduced into BamHI and XhoI sites of a pcDNA3.1 vector variant (pcDNA3.1(+)IRES GFP, a gift from Kathleen_L Collins; addgene plasmid#51406; http://n2t.net/addgene:51406; RRID:Addgene_51406). We replaced the neomycin resistance gene (NeoR) with the cDNA for Blasticidin S deaminase (bsd), amplified with forward primer bsd fwd and reverse primer bsd rev, by integration into the XmaI and BssHII sites of the vector. CD4 domain deletion mutants were generated using the Q5 Site-Directed Mutagenesis Kit (NEB) according to the manufactureŕs protocol. For mutants lacking domain 1 of hCD4 we introduced an N-terminal BC2-tag (43). For the generation of plasmid pcDNA3.1_CD4_ΔD1_IRES-eGFP we used forward primer ΔD1 fwd and reverse primer ΔD1 rev; for pcDNA3.1_CD4_ΔD1ΔD2_IRES-eGFP forward primer ΔD1ΔD2 fwd and reverse primer ΔD1ΔD2 rev; for pcDNA3.1_CD4_ΔD3ΔD4_IRES-EGFP forward primer ΔD3ΔD4 fwd and reverse primer ΔD3ΔD4 rev. For bacterial expression of Nbs, sequences were cloned into the pHEN6 vector (76), thereby adding a C-terminal sortase tag LPETG followed by 6xHis-tag for IMAC purification as described previously (42). For protein production of the extracellular domains 1-4 of hCD4 in Expi293 cells, corresponding cDNA was amplified from plasmid DNA containing full-length human CD4 cDNA (addgene plasmid #110192) using forward primer CD4-D1-4 f and reverse primer CD4-D1-4 r. A 6xHis tag was introduced by the reverse primer. Esp3I and EcoRI restriction sites were used to introduce the cDNA into a pcDNA3.4 expression vector with the signal peptide MGWTLVFLFLLSVTAGVHS from the antibody JF5 (77).
Cell culture, transfection, stable cell line generation
HEK293T and CHO-K1 cells were obtained from ATCC (CCL-61, LGC Standards GmbH, Germany). As this study does not include cell line-specific analysis, cells were used without additional authentication. Cells were cultivated according to standard protocols. Briefly, growth media containing DMEM (HEK293) or DMEM/F12 (CHO) (both high glucose, pyruvate, Thermo Fisher Scientific (TFS)) supplemented with 10% (v/v) FBS, L-glutamine and penicillin/streptomycin (P/S; all from TFS) were used for cultivation. Cells were passaged using 0.05% trypsin-EDTA (TFS) and were cultivated at 37°C and 5% CO2 atmosphere in a humidified chamber. Plasmid DNA was transfected using Lipofectamine 2000 (TFS) according to the manufacturer’s protocol. For the generation of the stable HEK293-hCD4 and CHO-hCD4 cell line, 24 h post transfection, cells were subjected to a two-week selection period using 5 µg/ml Blasticidin S (Sigma Aldrich) followed by single cell separation. Individual clones were analyzed by live-cell fluorescence microscopy regarding their level and uniformity of GFP and CD4 expression.
Protein expression and purification
CD4-specific Nbs were expressed and purified as previously published (74, 78). Extracellular fragment of human CD4 comprising domains 1-4 of human CD4 and a C-terminal His6-tag was expressed in Expi293 cells according to the manufactureŕs protocol (Thermo Fisher Scientific). Cell supernatant was harvested by centrifugation 4 days after transfection, sterile filtered and purified according to previously described protocols (79). For quality control, all purified proteins were analyzed via SDS-PAGE according to standard procedures. Therefore, protein samples were denaturized (5 min, 95°C) in 2x SDS-sample buffer containing 60 mM Tris/HCl, pH6.8; 2% (w/v) SDS; 5% (v/v) 2-mercaptoethanol, 10% (v/v) glycerol, 0.02% bromphenole blue. All proteins were visualized by InstantBlue Coomassie (Expedeon) staining. For immunoblotting proteins were transferred to nitrocellulose membrane (Bio-Rad Laboratories) and detection was performed using anti-His primary antibody (Penta-His Antibody, #34660, Qiagen) followed by donkey-anti-mouse secondary antibody labeled with AlexaFluor647 (Invitrogen) using a Typhoon Trio scanner (GE-Healthcare, excitation 633 nm, emission filter settings 670 nm BP 30).
Live-cell immunofluorescence
CHO-hCD4, and CHO wt cells transiently expressing CD4 domain-deletion mutants were plated at ∼10,000 cells per well of a µClear 96-well plate (Greiner Bio One, cat. #655090) and cultivated at standard conditions. Next day, medium was replaced by live-cell visualization medium DMEMgfp-2 (Evrogen, cat. #MC102) supplemented with 10% FBS, 2 mM L- glutamine, 2 µg/ml Hoechst33258 (Sigma Aldrich) for nuclear staining, and fluorescently labeled or unlabeled CD4-Nbs at concentrations between 1 nM and 100 nM. Unlabeled CD4- Nbs were visualized by addition of 2.5 µg/ml anti-VHH secondary Cy5 AffiniPure Goat Anti-Alpaca IgG (Jackson Immuno Research). Images were acquired with a MetaXpress Micro XL system (Molecular Devices) at 20× or 40× magnification.
Biolayer interferometry (BLI)
To determine the binding affinity of purified Nbs to recombinant hCD4, biolayer interferometry (BLItz, ForteBio) was performed. First, CD4 was biotinylated by 3-fold molar excess of biotin- N-hydroxysuccinimide ester. CD4 was then immobilized at single-use streptavidin biosensors (SA) according to manufacturer’s protocols. For each Nb we executed four association/dissociation runs with concentrations appropriate for the affinities of the respective nanobodies (overall between 15.6 nM and 1 µM). As a reference run, PBS was used instead of Nb in the association step. As negative control the GFP-Nb (500 nM) was applied in the binding studies. Recorded sensograms were analyzed using the BLItzPro software and dissociation constants (KD) were calculated based on global fits. For the epitope competition analysis, two consecutive application steps were performed, with a short dissociation period of 30 s after the first association.
PBMC isolation, cell freezing, and thawing
Fresh blood, buffy coats, or mononuclear blood cell concentrates were obtained from healthy volunteers at the Department of Immunology or from the ZKT Tübingen gGmbH. Participants gave informed consent and the studies were approved by the ethical review committee of the University of Tübingen, projects 156/2012B01 and 713/2018BO2. Blood products were diluted with PBS 1x (homemade from 10x stock solution, Lonza, Switzerland) and PBMCs were isolated by density gradient centrifugation with Biocoll separation solution (Biochrom, Germany). PBMCs were washed twice with PBS 1x, counted with a NC-250 cell counter (Chemometec, Denmark), and resuspended in heat-inactivated (h.i.) fetal bovine serum (Capricorn Scientific, Germany) containing 10% DMSO (Merck). Cells were immediately transferred into a -80°C freezer in a freezing container (Mr. Frosty; Thermo Fisher Scientific). After at least 24 hours, frozen cells were transferred into a liquid nitrogen tank and were kept frozen until use. For the experiments, cells were thawed in IMDM (+L-Glutamin +25mM HEPES; Life Technologies) supplemented with 2.5% h.i. human serum (HS; PanBiotech, Germany), 1x P/S (Sigma-Aldrich), and 50 µm β-Mercaptoethanol (β-ME; Merck), washed once, counted and used for downstream assays.
Affinity determination by flow cytometry
For cell-based affinity determination, HEK293-hCD4 were detached using enzyme-free cell dissociation buffer (Gibco) and resuspended in FACS buffer (PBS containing 5% FBS). For each staining condition 200,000 cells were incubated with suitable dilution series of CD4 nanobodies at 4°C for 30 min. Cells were washed two times and for detection Cy5 AffiniPure Goat Anti-Alpaca IgG, VHH domain (Jackson ImmunoResearch) was applied for 15 min. PBMCs (Department of Immunology/ ZKT Tübingen gGmbH, Germany) were freshly thawed and resuspended in FACS buffer. For each sample 200,000 cells were incubated with suitable concentrations of CD4 Nbs coupled to CF568 in combination with 1:500 dilution of anti-CD3- FITC (BD Biosciences) at 4°C for 30 min. For control staining PE/Cy5-labeled anti-human CD4 antibody (RPA-T4, Biolegend) was used. After two washing steps, samples were resuspended in 200 µl FACS buffer and analyzed with a BD FACSMelody Cell Sorter. Final data analysis was performed via FlowJo10® software (BD Biosciences).
Sortase labeling of nanobodies
Sortase A pentamutant (eSrtA) in pET29 was a gift from David Liu (Addgene plasmid # 75144) and was expressed and purified as described (80). CF568-coupled peptide H-Gly-Gly-Gly- Doa-Lys-NH2 (sortase substrate) was custom-synthesized by Intavis AG. For the click chemistry a peptide H-Gly-Gly-Gly-propyl-azide was synthesized. In brief, for sortase coupling 50 μM Nb, 250 μM sortase peptide dissolved in sortase buffer (50 mM Tris, pH 7.5, and 150 mM NaCl) and 10 μM sortase were mixed in coupling buffer (sortase buffer with 10 mM CaCl2) and incubated for 4 h at 4°C. Uncoupled Nb and sortase were depleted by IMAC. Unbound excess of unreacted sortase peptide was removed using Zeba Spin Desalting Columns (ThermoFisher Scientific, cat. #89890). Azide-coupled Nbs were labeled by SPAAC (strain- promoted azide-alkyne cycloaddition) click chemistry reaction with 2-fold molar excess of DBCO-Cy5.5 (Jena Bioscience) for 2 h at 25°C. Excess DBCO-Cy5.5 was subsequently removed by dialysis (GeBAflex-tube, 6-8 kDa, Scienova). Finally, to remove untagged Nb, (side product of the sortase reaction), we used hydrophobic interaction chromatography (HIC, HiTrap Butyl-S FF, Cytiva). Binding of DBCO-Cy5.5-coupled Nb occurred in 50 mM H2NaPO4, 1.5 M (NH4)2SO4, pH7.2. Elution took place with 50 mM H2NaPO4, pH7.2. Dye-labeled protein fractions were analyzed by SDS-PAGE followed by fluorescent scanning on a Typhoon Trio (GE-Healthcare, CF568: excitation 532 nm, emission filter settings 580 nm BP 30; Cy5.5 excitation 633 nm, emission filter settings 670 nm BP 30; 546) and subsequent Coomassie staining. Identity and purity of final products were determined by LC-MS (CD4-Nbs-CF568, >60%; CD4-Nb1-Cy5.5, ∼94%; CD4-Nb4-Cy5.5, ∼99%; GBP-Cy5.5; ∼94%, CD4-Nb1-3, ∼99%; bivGFP-Nb, ∼99%).
Hydrogen-deuterium exchange
CD4 deuteration kinetics and epitope elucidation
On basis of the affinity constants of 5.1 nM (CD4-Nb1), 6.5 nM (CD4-Nb2), 75.3 nM (CD4- Nb3) (pre-determined by BLI analysis) the molar ratio of antigen to Nb was calculated ensuring 90% complex formation according to (81). CD4 (5 µL, 65.5 µM) was pre-incubated with CD4- specific Nbs (5 µl; 60.3; 67.4 and 143.1 µM for Nb1; Nb2 and Nb3 respectively) for 10 min at 25°C. Deuteration samples containing CD4 only were pre-incubated with PBS instead of the Nbs. HDX of the pre-incubated samples was initiated by 1:10 dilution with PBS (150 mM NaCl, pH7.4) prepared with D2O leading to a final content of 90% D2O. After 5 and 50 min incubation at 25°C, aliquots of 20 µL were taken and quenched by adding 20 µL ice-cold quenching solution (0.2 M TCEP with 1.5% formic acid and 4 M guanidine HCl in 100 mM ammonium formate solution pH2.2) resulting in a final pH of 2.5. Quenched samples were immediately snap-frozen.
Immobilized pepsin (TFS) was prepared using 60 µl of 50% slurry (in ammonium formate solution pH2.5) that was then dried by centrifugation (1000 x g for 3 min at 0°C) and discarding the supernatant. Prior each analysis, samples were thawed and added to the dried pepsin beads. After digestion for 2 min in a water ice bath the samples were separated by centrifugation at 1000 x g for 30 s at 0°C using a 22 µm filter (Merck, Millipore) and were immediately analyzed by LC-MS. Undeuterated control samples for each complex and CD4 alone were prepared under the same conditions using H2O instead of D2O. Additionally, each Nb was digested without addition of CD4 to generate a list of peptic peptides deriving from the Nb. The HDX experiments of the CD4-Nb-complex were performed in triplicates. The back- exchange of the method as determined using a standard peptide mixture of 14 synthetic peptides was 24%.
Chromatography and Mass Spectrometry
HDX samples were analyzed as described previously (78)
HDX data analysis
A peptic peptide list was generated in a preliminary LC-MS/MS experiment as described previously (78). For data based search no enzyme selectivity was applied, furthermore, identified peptides were manually evaluated to exclude peptides originated through cleavage after arginine, histidine, lysine, proline and the residue after proline (82). Additionally, a separate list of peptides for each nanobody was generated and peptides overlapping in mass, retention time and charge with the antigen digest, were manually removed. Analysis of the deuterated samples was performed in MS mode only and HDExaminer v2.5.0 (Sierra Analytics, USA) was used to calculate the deuterium uptake (centroid mass shift). HDX could be determined for peptides covering 87-88% of the CD4 sequence (Supplementary Fig. 11). The calculated percentage deuterium uptake of each peptide between CD4-Nb and CD4-only were compared. Any peptide with uptake reduction of 5% or greater upon Nb binding was considered as protected. All relevant HDX parameters are shown in Supplementary Table S3 as recommended (83).
Endotoxin determination and removal
The concentration of bacterial endotoxins was determined with Pierce LAL Chromogenic Endotoxin Quantitation Kit (Thermo Fisher Scientific) and removal occurred using EndoTrap HD 1 ml (Lionex) according to the manufacturerś protocols.
Synthetic peptides
The following HLA-class II peptides were used for the stimulations: MHC class II pool (HCMVA pp65 aa 109-123 MSIYVYALPLKMLNI, HCMV pp65 aa 366-382 HPTFTSQYRIQGKLEYR, EBVB9 EBNA2 aa 276-290 PRSPTVFYNIPPMPL, EBVB9 EBNA1 aa 514-527 KTSLYNLRRGTALA, EBV BXLF2 aa 126-140 LEKQLFYYIGTMLPNTRPHS, EBV BRLF1 aa 119-133 DRFFIQAPSNRVMIP, EBVB9 EBNA3 aa 381-395 PIFIRRLHRLLLMRA, EBVB9 GP350 aa 167-181 STNITAVVRAQGLDV, IABAN HEMA aa 306-318 PKYVKQNTLKLAT,) or CMVpp65 aa 510-524 YQEFFWDANDIYRIF. All peptides were synthesized and dissolved in water 10% DMSO as previously described (purity ≥ 80%), and were kindly provided by S. Stevanović (84).
Stimulation and cultivation of PBMCs
PBMCs from donors previously screened for ex vivo CD4+ T cell reactivities against MHC- class II peptides were thawed and rested in T cell medium (TCM; IMDM + 1x P/S + 50μM β- ME + 10% h.i. HS) containing 1μg/mL DNase I (Sigma-Aldrich) at a concentration of 2-3x106 cells/mL for 3h at 37°C and 7.5% CO2. After resting, cells were washed once, counted and up to 1x108 cells were labeled with 1.5-2 μM Carboxyfluorescein succinimidyl ester (CFSE; BioLegend, USA) in 1 mL PBS 1X for 20 min according to the manufacturer’s protocol. The cells were washed twice in medium containing 10% FBS after CFSE labeling and incubated with 5 μM, 0.5 μM, or 0.05 μM of CD4-Nb1, CD4-Nb4 or a control Nb for 1h at 37°C in serum-free IMDM medium. Concentrations and duration were chosen to mimick the expected approximate concentration and serum retention time during clinical application. After incubation, cells were washed twice, counted and each condition was separated into three parts and seeded in a 48-well cell culture plate (1.6-2.5x106 cells/well in triplicates). Cells were stimulated with either 10 μg/ml PHA-L (Sigma-Aldrich), 5 μg/mL MHC class-II peptide(s) or left unstimulated, and cultured at 37°C and 7.5% CO2. 2 ng/mL recombinant human IL-2 (R&D, USA) were added on days 3, 5, and 7. One third of the culture on day 4, one half of the culture on day 6 and day 8, and the remaining cells on day 12 were harvested, counted and stained for flow cytometry analyses. For donor 1, the proliferation/activation status and cytokine production were analyzed in two different experiments, whereas for donors 2 and 3, cells from a single experiment were used for the three assays.
Assessment of T cell proliferation and activation
Cells from days 4, 6, and 8 were transferred into a 96-well round-bottom plate and washed twice with FACS buffer (PBS + 0.02% sodium azide (Roth, Germany) +2 mM EDTA (Sigma- Aldrich) +2% h.i. FBS). Extracellular staining was performed with CD4 APC-Cy7 (RPA-T4, BD Biosciences), CD8 BV605 (RPA-T8, BioLegend), the dead cell marker Zombie Aqua (BioLegend), CD25 PE-Cy7 (BC96, BioLegend), CD69 PE (FN50, BD Biosciences) and incubated for 20 min at 4°C. All antibodies were used at pre-tested optimal concentrations. Cells were washed twice with FACS buffer. Approx. 500.000 cells were acquired on the same day using a LSRFortessaTM SORP (BD Biosciences, USA) equipped with the DIVA Software (Version 6, BD Biosciences, USA). The percentage of proliferating CD4+ cells was determined by assessment of CFSE negative cells, activation by the percentage of CD69+ or CD25+.
Assessment of T cell function by intracellular cytokine staining
On day 12, the MHC class II peptide(s)-stimulated and cultured cells were transferred into a 96-well round-bottom plate (0.5 to 1x 106 cells/well) and restimulated using 10 µg/ml of the same peptide(s), 10 µg/ml Staphylococcus enterotoxin B (SEB, Sigma-Aldrich; positive control), or 10% DMSO (negative control). Protein transport inhibitors Brefeldin A (10 µg/ml, Sigma-Aldrich) and Golgi Stop (BD Biosciences) were added at the same time as the stimuli. After 14 h stimulation at 37°C and 7.5% CO2, cells were stained extracellularly with the fluorescently labeled antibodies CD4 APC-Cy7, CD8 BV605, and Zombie Aqua and incubated for 20 min at 4°C. After, cells were washed once, then fixed and permeabilized using the BD Cytofix/Cytoperm solution (BD Biosciences) according to the manufacturer’s instructions, stained intracellularly with TNF Pacific Blue (Mab11), IL-2 PE-Cy7 (MQ1-17H12), IFN-γ AlexaFluor 700 (4S.B7) and CD154 APC (2431) antibodies (all BioLegend) (85) and washed twice. Approx. 500,000 cells were acquired on the same day using a LSRFortessaTM SORP (BD Biosciences, USA), equipped with the DIVA Software (Version 6, BD Biosciences). All flow cytometry analyses were performed with FlowJo version 10.6.2, gating strategies are shown in Supplementary Fig. 6. Statistical analyses were performed with GraphPad Prism version 9.0.0.
Full blood stimulation and cytokine release assay
100 μl of lithium-heparin blood was incubated for 1 h at 37°C and 7.5% CO2. The blood was stimulated with 5 μM Nb (CD4-Nb1, CD4-Nb4 or control Nb), with 100 ng/mL LPS (Invivogen, USA), or with 2 μg/mL PHA-L in a final volume of 250 μl (serum-free IMDM medium), or left unstimulated for 24 h at 37°C and 7.5% CO2. After two centrifugations, supernatant was collected without transferring erythrocytes. The supernatants were frozen at -80°C until cytokine measurements. Levels of IL-1β, IL-1Ra, IL-4, IL-6, IL-8, IL-10, IL-12p70, IL-13, GM- CSF, IFNγ, MCP-1, MIP-1β, TNFα and VEGF were determined using a set of in house developed Luminex-based sandwich immunoassays each consisting of commercially available capture and detection antibodies and calibrator proteins. All assays were thoroughly validated ahead of the study with respect to accuracy, precision, parallelism, robustness, specificity and sensitivity (86, 87). Samples were diluted at least 1:4 or higher. After incubation of the pre- diluted samples or calibrator protein with the capture coated microspheres, beads were washed and incubated with biotinylated detection antibodies. Streptavidin-phycoerythrin was added after an additional washing step for visualization. For control purposes, calibrators and quality control samples were included on each microtiter plate. All measurements were performed on a Luminex FlexMap® 3D analyzer system, using Luminex xPONENT® 4.2 software (Luminex, USA). For data analysis MasterPlex QT, version 5.0 was employed. Standard curve and quality control samples were evaluated according to internal criteria adapted to the Westgard Rules (88) to ensure proper assay performance.
Analysis of cross-species reactivity binding to mouse CD4+ cells by flow cytometry
Murine CD4+ cells were isolated from spleen and lymph nodes of C57BL/6N mice by positive selection over CD4 magnetic microbeads (Miltenyi Biotech, Germany). Human CD4+ cells were extracted from blood using StraightFrom® Whole Blood CD4 MicroBeads (Miltenyi Biotech). Single cell suspensions were incubated with 0.75 µg/ml of CD4-Nbs-Cy5.5 (∼47 – 60 nM) or GFP-Nb-Cy5.5 (∼51 nM) in 1% FPS/PBS at 4°C for 20 min and subsequently analyzed on a LSR-II cytometer (BD biosciences).
Optical Imaging of CD4-expressing HPB-ALL tumors
Human T cell leukemia HPB-ALL cells (German Collection of Microorganisms and Cell Cultures GmbH, DSMZ, Braunschweig, Germany) were cultured in RPMI-1640 supplemented with 10% FBS and 1% P/S. 107 HPB-ALL cells were injected subcutaneously in the right upper flank of 7-week-old NOD SCID gamma mice (NSG, NOD.Cg-Prkdcscid Il2rgtm1WjI/SzJ, Charles River Laboratories, Sulzfeld, Germany) and tumor growth was monitored for 2-3 weeks. When tumors reached a diameter ∼7 mm, 5 µg of CD4-Nbs-Cy5.5 or control Nb (GFP-Nb-Cy5.5) were administered into the tail vein of 2 mice each. Optical imaging (OI) was performed repetitively in short-term isoflurane anesthesia over a period of 24 h using the IVIS Spectrum In Vivo Imaging System (PerkinElmer, Waltham, MA, USA). Four days after the first Nb administration, the CD4-Nbs-Cy5.5 groups received the GFP-Nb-Cy5.5 (and vice versa) and tumor biodistribution was analyzed identically by OI over 24 h. After the last imaging time point, animals were sacrificed and tumors were explanted for ex vivo OI analysis. Data were analyzed with Living Image 4.4 software (PerkinElmer). The fluorescence intensities were quantified by drawing regions of interest around the tumor borders and were expressed as average radiant efficiency (photons/s)/(μW/cm2) subtracted by the background fluorescence signal before Nb injection to eliminate potential residual signal from the previous Nb application. All mouse experiments were performed according to the German Animal Protection Law and were approved by the local authorities (Regierungspräsidium Tübingen, R5/18).
Immunofluorescence staining of explanted xenograft tumors
Freshly frozen 5 µm sections of hCD4-Nb1-Cy5.5-containing mice tumors were analyzed using an LSM 800 laser scanning microscope (Zeiss). Afterwards the sections were fixed with perjodate-lysine-paraformaldehyde, blocked using donkey serum and stained with primary rabbit-anti-CD4 antibody (Cell Marque, USA). Bound antibody was visualized using donkey- anti-rabbit-Cy3 secondary antibody (Dianova, Germany). YO-PRO-1 (Invitrogen, USA) was used for nuclear staining. Acquired images of the same areas were manually overlaid.
Analyses and Statistics
Data analysis of the flow cytometry data was performed with the FlowJo Software Version 10.6.2 (FlowJo LLT, USA) and graph preparation and statistical analysis was performed using the GraphPad Prism Software (Version 8.3.0 or higher).
Supplementary Information
Supplementary Methods
Acknowledgements
This work received financial support from the State Ministry of Baden-Wuerttemberg for Economic Affairs, Labour and Tourism (Grant: Predictive diagnostics of immune-associated diseases for personalized medicine. FKZ: 35-4223.10/8). The authors thank Sandra Maier and Ulrich Kratzer (both Natural and Medical Sciences Institute at the University of Tuebingen) for technical support with MS analyses, and Birgit Fehrenbacher (Department of Dermatology, University of Tuebingen) for technical support with imaging of xenograft cryosections.
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