Amit Novik

The interaction of TIGIT with PVR and PVRL2 inhibits human NK cell cytotoxicity

NK cell cytotoxicity is controlled by numerous NK inhibitory and activating receptors. Most of the inhibitory receptors bind MHC class I proteins and are expressed in a variegated fashion. It was recently shown that TIGIT, a new protein expressed by T and NK cells binds to PVR and PVR-like receptors and inhibits T cell activity indirectly through the manipulation of DC activity. Here, we show that TIGIT is expressed by all human NK cells, that it binds PVR and PVRL2 but not PVRL3 and that it inhibits NK cytotoxicity directly through its ITIM. Finally, we show that TIGIT counter inhibits the NK-mediated killing of tumor cells and protects normal cells from NK-mediated cytoxicity thus providing an “alternative self” mechanism for MHC class I inhibition.

Peptides modulating conformational changes in secreted chaperones: From in silico design to preclinical proof of concept

Blocking conformational changes in biologically active proteins holds therapeutic promise. Inspired by the susceptibility of viral entry to inhibition by synthetic peptides that block the formation of helix–helix interactions in viral envelope proteins, we developed a computational approach for predicting interacting helices. Using this approach, which combines correlated mutations analysis and Fourier transform, we designed peptides that target gp96 and clusterin, 2 secreted chaperones known to shift between inactive and active conformations. In human blood mononuclear cells, the gp96-derived peptide inhibited the production of TNFα, IL-1β, IL-6, and IL-8 induced by endotoxin by >80%. When injected into mice, the peptide reduced circulating levels of endotoxin-induced TNFα, IL-6, and IFNγ by >50%. The clusterin-derived peptide arrested proliferation of several neoplastic cell lines, and significantly enhanced the cytostatic activity of taxol in vitro and in a xenograft model of lung cancer. Also, the predicted mode of action of the active peptides was experimentally verified. Both peptides bound to their parent proteins, and their biological activity was abolished in the presence of the peptides corresponding to the counterpart helices. These data demonstrate a previously uncharacterized method for rational design of protein antagonists.

Genomic fossils as a snapshot of the human transcriptome

Processed pseudogenes (PPGs) are cDNA sequences that were generated through reverse transcription of mature, spliced mRNAs and have subsequently been reinserted at a new genomic location. These cDNA sequences are usually no longer transcribed and are considered “dead on arrival.” Here we show that PPGs can be used to generate a map of the transcriptome. By analyzing thousands of human PPGs, we were able to discover hundreds of transcript variants so far unidentified. An experimental verification of a subset of these variants by RT-PCR indicates that most of them are still active in the human transcriptome. Furthermore, we demonstrate that PPGs can enable the identification of ancient splice variants that were expressed ancestrally but are now extinct. Our results show that the genome itself carries a “virtual cDNA library” that can readily be used to analyze both present and ancestral transcripts. Our approach can be applied to sequenced metazoan genomes to computationally annotate splicing variation even when expressed sequences are unavailable.

Evolution of multicellularity in Metazoa: comparative analysis of the subcellular localization of proteins in Saccharomyces, Drosophila and Caenorhabditis

A comparison of the subcellular assignments of proteins between the unicellular Saccharomyces cerevisiae and the multicellular Drosophila melanogaster and Caenorhabditis elegans was performed using a computational tool for the prediction of subcellular localization. Nine subcellular compartments were studied: (1) extracellular domain, (2) cell membrane, (3) cytoplasm, (4) endoplasmic reticulum, (5) Golgi apparatus, (6) lysosome, (7) peroxisome, (8) mitochondria, and (9) nucleus. The transition to multicellularity was found to be characterized by an increase in the total number of proteins encoded by the genome. Interestingly, this increase is distributed unevenly among the subcellular compartments. That is, a disproportionate increase in the number of proteins in the extracellular domain, the cell membrane, and the cytoplasm is observed in multicellular organisms, while no such increase is seen in other subcellular compartments.

Activation of Relaxin‐Related Receptors by Short, Linear Peptides Derived from a Collagen‐Containing Precursor

In a screening effort based on algorithmic predictions for novel G‐protein‐coupled receptor (GPCR) peptide activators, we were able to identify and examine two novel peptides (P59 and P74) which are short, linear, and derived from a natural, previously unidentified precursor protein containing a collagen‐like repeat. Both peptides seemed to show an apparent cAMP‐related effect on CHO‐K1 cells transiently transfected with either LGR7 or LGR8, usually after treatment with cAMP‐generating forskolin, compared to the same cells treated with forskolin plus relaxin. This activation was not found for the relaxin‐3 receptor (GPR135). In a set of follow‐up experiments, both peptides were found to stimulate cAMP production, mostly upon initial stimulation of cAMP production by 5 μM forskolin in cells transfected with either LGR7 or LGR8. In a dye‐free cell impedance GPCR activation assay, we were able to show that these peptides were also able to activate a cellular response mediated by these receptors. Although untransfected CHO‐K1 cells showed some cellular activation by both relaxin and at least one of our newly discovered peptides, both LGR7‐ and LGR8‐transfected cells showed a stronger response, indicating stimulation of a cellular pathway through activation of these receptors. In conclusion, we were able to show that these newly discovered peptides, which have no similarity to any member of the relaxin–insulin‐like peptide family, are potential ligands for the relaxin‐related family of receptors and as such might serve as novel candidates for relaxin‐related therapeutic indications. Both peptides are linear and were found to be active after being chemically synthesized.

Follow the leader: preference for specific amino acids directly following the initial methionine in proteins of different organisms.

It is well established that the vast majority of proteins of all taxonomical groups and species are initiated by an AUG codon, translated into the amino acid methionine (Met). Many attempts were made to evaluate the importance of the sequences surrounding the initiation codon, mostly focusing on the RNA sequence. However, the role and importance of the amino acids following the initiating Met residue were rarely investigated, mostly in bacteria and fungi. Herein, we computationally examined the protein sequences of all major taxonomical groups represented in the Swiss-Prot database, and evaluated the preference of each group to specific amino acids at the positions directly following the initial Met. The results indicate that there is a species-specific preference for the second amino acid of the majority of protein sequences. Interestingly, the preference for a certain amino acid at the second position changes throughout evolution from lysine in prokaryotes, through serine in lower eukaryotes, to alanine in higher plants and animals.

ILDR2 Is a Novel B7-like Protein That Negatively Regulates T Cell Responses

The B7-like protein family members play critical immunomodulatory roles and constitute attractive targets for the development of novel therapies for human diseases. We identified Ig-like domain–containing receptor (ILDR)2 as a novel B7-like protein with robust T cell inhibitory activity, expressed in immune cells and in immune-privileged and inflamed tissues. A fusion protein, consisting of ILDR2 extracellular domain with an Fc fragment, that binds to a putative counterpart on activated T cells showed a beneficial effect in the collagen-induced arthritis model and abrogated the production of proinflammatory cytokines and chemokines in autologous synovial-like cocultures of macrophages and cytokine-stimulated T cells. Collectively, these findings point to ILDR2 as a novel negative regulator for T cells, with potential roles in the development of immune-related diseases, including autoimmunity and cancer.

ILDR2-Fc Is a Novel Regulator of Immune Homeostasis and Inducer of Antigen-Specific Immune Tolerance

ILDR2 is a member of the Ig superfamily, which is implicated in tricellular tight junctions, and has a putative role in pancreatic islet health and survival. We recently found a novel role for ILDR2 in delivering inhibitory signals to T cells. In this article, we show that short-term treatment with ILDR2-Fc results in long-term durable beneficial effects in the relapsing-remitting experimental autoimmune encephalomyelitis and NOD type 1 diabetes models. ILDR2-Fc also promotes transplant engraftment in a minor mismatch bone marrow transplantation model. ILDR2-Fc displays a unique mode of action, combining immunomodulation, regulation of immune homeostasis, and re-establishment of Ag-specific immune tolerance via regulatory T cell induction. These findings support the potential of ILDR-Fc to provide a promising therapeutic approach for the treatment of autoimmune diseases.

Abstract B291: Identification of novel immune checkpoints and their implementation as mAb targets for cancer immunotherapy.

Immune checkpoints, such as CTLA4 and PD-1, have emerged as promising drug targets for cancer immunotherapy. We hypothesize that additional novel members of the B7/CD28 family play a role in T cell regulation and thus may serve as targets for therapeutic mAbs. However, the discovery of novel family members is challenging since proteins of the immune system, including proteins of the B7 protein In order to identify novel members of the B7/CD28 protein family, Compugen has developed a discovery approach integrating gene and protein information with extensive expression data, and has identified nine novel membrane proteins that possess characteristics of the B7/CD28 protein family members and are therefore predicted to play a role in T cell co-stimulation. In order to validate our predictive discovery findings, we evaluated the effect of our proteins on immune cells, particularly T cells. For that goal, we expressed the proteins on the cell surface upon ectopic expression, and also produced fusion proteins consisting of the extracellular domain of the predicted proteins, fused to an IgG Fc domain. Here we present results obtained for two of our novel proteins, CGEN-15001T and CGEN-15022. Both display robust inhibition of T cell activation. Interestingly, CGEN-15001, one of the Fc-fused proteins, leads to increased levels of anti-inflammatory cytokines such as IL-4 and IL5, while reducing pro-inflammatory cytokines such as IFN-γ and IL-17. In addition, CGEN-15001 was found to enhance iTregs differentiation. Furthermore, these molecules showed therapeutic efficacy in mouse models of multiple sclerosis and rheumatoid arthritis. To investigate the potential of these membrane proteins as drug targets for treatment of cancer we have performed extensive IHC studies, on a variety of healthy and malignant tissues. Both CGEN-15001T and CGEN-15022 were found to be expressed in numerous types of cancers, each showing a unique pattern of expression. CGEN-15001T, in addition to its expression on tumor cells, was found to be expressed on tumor infiltrating immune cells, especially on Macrophages and Mast cells. Based on the immunomodulatory activities and the expression pattern on malignant and immune cells, CGEN15001T and CGEN15022 may serve as mAb targets for cancer immunotherapy. Citation Information: Mol Cancer Ther 2013;12(11 Suppl):B291. Citation Format: Gady Cojocaru, Ofer Levy, Amir Toporik, Liat Dassa, Iris Hecht, Ilan Vaknin, Sergey Nemzer, Tania Pergan, Amit Novik, Shirley Sameah-Greenwald, Anat Oren, Zohar Tiran, Peter Steinberger, Joseph Podojil, Nora Tarcic, Eyal Neria, Galit Rotman, Zurit Levine. Identification of novel immune checkpoints and their implementation as mAb targets for cancer immunotherapy. [abstract]. In: Proceedings of the AACR-NCI-EORTC International Conference: Molecular Targets and Cancer Therapeutics; 2013 Oct 19-23; Boston, MA. Philadelphia (PA): AACR; Mol Cancer Ther 2013;12(11 Suppl):Abstract nr B291.

Peptides modulating conformational changes: From in silico design to in vivo proof of concept

From in-Silico Design to in-Vivo Proof of Concept Yossef Kliger, Ofer Levy, Anat Oren, Haim Ashkenazy, Zohar Tiran, Amit Novik, Avi Rosenberg, Anat Amir, Assaf Wool, Amir Toporik, Ehud Schreiber, Dani Eshel, Zurit Levine, Yossi Cohen, Claudia Nold-Petry, Charles A. Dinarello, Itamar Borukhov 1Compugen Ltd. Tel Aviv 69512, Israel. (www.cgen.com) *Correspondence: kliger@cgen.com, itamarb@cgen.com 2The Mina and Everard Goodman Faculty of Life Sciences, Bar Ilan University, Ramat Gan, Israel 3University of Colorado Denver, Aurora, CO 80045, USA