Modulation of insulin-like growth factor-1 receptor and its signaling network for the treatment of cancer: current status and future perspectives.

Based on over three decades of pre-clinical data, insulin-like growth factor-1 receptor (IGF-1R) signaling has gained recognition as a promoter of tumorogenesis, driving cell survival and proliferation in multiple human cancers. As a result, IGF-1R has been pursued as a target for cancer treatment. Early pioneering efforts targeting IGF-1R focused on highly selective monoclonal antibodies, with multiple agents advancing to clinical trials. However, despite some initial promising results, recent clinical disclosures have been less encouraging. Moreover, recent studies have revealed that IGF-1R participates in a dynamic and complex signaling network, interacting with additional targets and pathways thereof through various crosstalk and compensatory signaling mechanisms. Such mechanisms of bypass signaling help to shed some light on the decreased effectiveness of selective IGF-1R targeted therapies (e.g. monoclonal antibodies) and suggest that targeting multiple nodes within this signaling network might be necessary to produce a more effective therapeutic response. Additionally, such findings have led to the development of small molecule IGF-1R inhibitors which also co-inhibit additional targets such as insulin receptor and epidermal growth factor receptor. Such findings have helped to guide the design rationale of numerous drug combinations that are currently being evaluated in clinical trials.

Biology around type I insulin-like growth factor receptor signaling and its role in cancer

Type I insulin-like growth factor receptor (IGF-1R) is a receptor tyrosine kinase that plays an important role in promoting tumor cell survival and growth. Early evidence demonstrated that IGF-1R is required for cellular transformation, and expression of IGF ligands is linked to a number of tumor types including breast and colon.[1-3] During the past two decades, the importance of IGF-1R in cancer has been reinforced by pre-clinical studies showing that IGF-1R is an important driver of tumorogenesis, cell survival and proliferation in multiple human cancers including hepatocellular carcinoma (HCC), Ewing’s sarcoma, multiple myeloma, non-small cell lung carcinoma (NSCLC), and ovarian carcinoma.[4-6] Overexpression of the IGF-1R ligands IGF-I and IGF-II has been observed in various human cancers and is associated with increased disease incidence, progression and poor prognosis.[7,8] IGF-1R mediates these cancerpromoting properties through activation of two well established oncogenic pathways: the phosphatidylinositol-3-kinase (PI3K)/protein kinase B (Akt/PKB) pathway and the mitogen-activated protein kinases (MAPK) pathway.[9] The importance of IGF-1R signaling for the treatment of cancer is further underscored by the potential for IGF-1R signaling to promote resistance to both cytotoxic chemotherapies and radiation, as well as other molecular targeted therapies (Figure 1).[10-12]

Figure 1.

The insulin-like growth factor 1 receptor (IGF-1R), a transmembrane receptor tyrosine kinase, is activated by its cognate ligands, insulin-like growth factor-1 (IGF-1) and -2 (IGF-2), resulting in receptor auto-transphosphorylation and signaling cascades that progress through the IRS-l/PI3K/AKT and MAPK pathways. Stimulation of both pathways ultimately leads to various cancer promoting phenotypes including cellular proliferation, survival, invasion, metastasis and angiogenesis. Specific IGF-1R mediated activation of the PI3K/AKT pathway results in a pro-survival signal that has been shown to promote resistance to both chemotherapy-induced apoptosis or to molecular targeted therapies (Target X).

Based on pre-clinical data highlighting the critical role that IGF-1R plays in human cancer, major research efforts have been undertaken during the last decade, focused on discovering and developing therapeutic agents to modulate IGF-1R activity. These efforts have resulted in IGF-1R inhibitors that operate through several distinct modes of inhibition. These include monoclonal antibodies (mAbs) that neutralize the IGF-1R ligands IGF-1 and/or IGF-2 (e.g. dusigitumab, MEDI-573, an agent in this class that is currently being evaluated in clinical trials. ClinicalTrial.gov Identifiers: NCT01498952, NCT01446159), monoclonal antibodies that specifically target the IGF-1R extracellular ligand-binding domain, and small molecule inhibitors that target the IGF-1R intracellular catalytic domain. The third approach is further stratified into adenosine triphosphate (ATP) competitive inhibitors that bind to the ATP pocket of the IGF-1R kinase domain, and non-ATP competitive inhibitors that bind to an allosteric pocket (e.g. substrate binding site). Several excellent reviews have been published in recent years describing the historical developments in these areas.[13-15] This review will cover recently disclosed pre-clinical agents and provide an update on the current clinical landscape targeting IGF-1R. Furthermore, this review will discuss the evolution that has taken place in cancer biology surrounding IGF-1R signaling, from the initial static view of a single target in an isolated pathway to the current view of a dynamic landscape encompassing multiple targets and pathways interacting through a complex signaling network. Such a dynamic signaling network highlights the need for combination therapies for IGF-1R inhibitors in order to provide maximal benefit in the oncology setting.

Initial effort to develop selective type I insulin-like growth factor receptor inhibitors over insulin receptor

Type I insulin-like growth factor receptor specific monoclonal antibodies

One of the major concerns during the initial discovery and development of IGF-1R inhibitors centered around potential toxicity which was speculated to arise from targeting the highly homologous insulin receptor (IR). The IR supports critical physiological functions in regulating glucose homeostasis and, therefore, inhibition of IR could potentially lead to undesired toxicities such as hyperglycemia and hyperinsulinemia. Due to these concerns, mAbs that target the IGF-1R extra-cellular ligand-binding domain became a major focus since this recognition epitope is differentiated between IGF-1R and IR. Multiple IGF-1R mAb agents have been developed and have entered into clinical trials, including figitumumab (CP-751,871). Although the early disclosures for figitumumab reported encouraging clinical response,[16] two phase III trials evaluating figitumumab in NSCLC, NCT00596830 (figitumumab in combination with paclitaxel and carboplatin) and NCT00673049 (figitumumab in combination with erlotinib) were discontinued in 2010 as independent data analysis indicated both trials were unlikely to meet the primary end points. It should be pointed out that insulin resistance and hyperglycemia are observed as side effects in human clinical trials with figitumumab, presumably through a growth hormone-related mechanism, indicating that disturbances in glucose homeostasis can occur even through IGF-1R specific targeting.[17,18] Some data emerging from clinical studies with other IGF-1R neutralizing antibodies are also discouraging. For example, Amgen recently disclosed that a phase III trial evaluating their IGF-1R antibody AMG479 (ganitumab) in pancreatic cancer did not meet the primary end point. We are currently awaiting the results from a number of other clinical trials, single agent and combination, evaluating IGF-1R mAbs. These ongoing clinical activities are summarized in Table 1.

Table 1.

Insulin-like growth factor 1 receptor monoclonal antibodies: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R mAbs	In combination with	Phase	Indication	Trial ID
AMG 479 (Ganitumab)	—	II	Epithelial ovarian cancer	NCT00718523
	—	II	Recurrent platinum sensitive ovarian cancer	NCT00719212
	—	II	Ewing’s family tumor and desmoplastic small round cell tumors	NCT00563680
	—	II	Neuroendocrine tumor, carcinoid tumor, pancreatic neuroendocrine tumor	NCT01024387
	Gemcitabine, radiation, capecitabine	I	Locally advanced cancer of the pancreas	NCT01298401
	Everolimus	I	Advanced solid tumors	NCT01122199
	Everolimus, panitumumab	I	Advanced solid tumors	NCT01061788
	Platinum-based chemotherapy	Ib/II	Extensive stage small cell lung cancer	NCT00791154
	MEK162	Ib/II	Selected advanced solid tumors	NCT01562899
	Panitumumab	II	Colorectal cancer	NCT00788957
	Panitumumab	II	Wt K-Ras metastatic colorectal cancer	NCT00891930
	Metformin	II	Breast cancer	NCT01042379
	FOLFIRI	II	KRAS-mutant metastatic colorectal cancer	NCT00813605
IMC-A12 (Cixutumumab)	—	I	Solid tumors	NCT01007032
	—	II	Solid tumors	NCT00831844
	—	II	Mesothelioma	NCT01160458
	—	II	Thymoma, thymic carcinoma	NCT00965250
	—	II	Metastatic melanoma of the eye	NCT01413191
	—	II	Metastatic prostate cancer	NCT00520481
	Sorafenib	I	Hepatocellular carcinoma	NCT01008566
	Temozolomide, multi-agent chemotherapy	I	Metastatic rhabdomyosarcoma	NCT01055314
	Everolimus, octreotide acetate	I	Neuroendocrine carcinoma	NCT01204476
	Gemcitabine, Erlotinib	I/II	Metastatic pancreatic cancer	NCT00617708
	Temsirolimus	I/II	Metastatic prostate cancer	NCT01026623
	Temsirolimus	I/II	Locally recurrent or metastatic breast cancer	NCT00699491
	Doxorubicin	I/II	Soft tissue sarcoma	NCT00720174
	Sorafenib	II	Hepatocellular carcinoma	NCT00906373
	Temsirolimus	II	Metastatic sarcomas	NCT01016015
	Temsirolimus	II	Advanced cancers	NCT00678769
	Bicalutamide, goserelin, leuprolide acetate	II	Metastatic prostate cancer	NCT01120236
	Paclitaxel, carboplatin, bevacizumab	II	Non-small cell lung cancer	NCT00955305
	Cisplatin, pemetrexed	II	Non-small cell lung cancer	NCT01232452
	Carboplatin, pemetrexed	II	Non-small cell lung cancer	NCT01263782
	Antiestrogens	II	Breast cancer	NCT00728949
	Octreotide acetate	II	Metastatic neuroendocrine tumors	NCT00781911
	Mitotane	II	Adrenocortical carcinoma	NCT00778817
	Capecitabine, lapatinib	II	HER2 positive breast cancer	NCT00684983
	Cisplatin, etoposide	II	Extensive stage small cell lung cancer	NCT00887159
	Temsirolimus	II	Pediatric patients with recurrent or refractory solid tumors	NCT01614795
	Cisplatin, etoposide	II	Extensive stage small cell lung cancer	NCT00887159
	Cetuximab	II	Head and neck squamous cell carcinoma	NCT00957853
MK-0646 (Dalotuzumab)	Ridaforolimus	I	Advanced cancers	NCT01243762
	Ridaforolimus	I	Advanced solid tumors	NCT01431547
	Gemcitabine, erlotinib	I/II	Advanced pancreatic cancer	NCT00769483
	Pemetrexed, cisplatin	II	Metastatic non-squamous lung cancer	NCT00799240
	Ridaforolimus	II	Estrogen receptor positive breast cancer	NCT01234857
	Irinotecan	II	Metastatic rectal carcinoma	NCT01609231
	Ridaforolimus, exemestane	II	Breast cancer	NCT01605396
R1507	—	II	Ewing’s sarcoma, osteosarcoma, synovial sarcoma, rhabdomyosarcoma and other sarcomas	NCT00642941
	12 standard chemo drugs	I	Advanced malignancies	NCT00811993
	Everolimus	I	Advanced solid tumors	NCT00985374
SCH 717454 (Robatumumab)	—	II	Osteosarcoma sarcoma, Ewing’s peripheral neuroectodermal tumor	NCT00617890
MM-141	—	I	Advanced solid tumors	NCT01733004

IGF-1R, insulin-like growth factor 1 receptor; mAbs, monoclonal antibodies.

Efforts to develop small molecule type I insulin-like growth factor receptor inhibitors selective over insulin receptor

Discovery of small molecule inhibitors selectively targeting the IGF-1R intracellular kinase domain over IR has proven to be challenging, due to an overall protein sequence homology of 84% and an ATP binding pocket sequence homology of 100% between these two family members. Nonetheless, several compounds have been reported with more than 10-fold selectivity for IGF-1R over IR in specific mechanistic assays. As highlighted in Figure 2, compound 1a (NVP-AEW541), a pyrrolo[2,3-d]pyrimidine derivative, was reported to inhibit IGF-IR in cells (cellular IC50=0.086 M) with ~27-fold selectivity versus IR (cellular IC50=2.3 M), despite the observed equal potency versus IGF-1R and IR in biochemical assays. The selectivity achieved was attributed to subtle conformational differences between the two receptors in the cellular setting along with the fact that the biochemical assay employed only the truncated kinase domain of each receptor. Compound 1a significantly reduces the growth of IGF-IR-driven fibrosarcomas and demonstrated in vivo tumor growth inhibition (TGI) in xenograft models.[19] Very recently, it was reported that compound 1a enhances the effect of ionizing radiation in PTEN wild-type, but not in PTEN-deficient, prostate cancer cells.[20] Compound 1b (NVP-ADW742), a close analog of 1a, was also disclosed with a 16-fold selectivity window for IGF-1R over IR in the cellular setting.[21] Compounds 1a and 1b were the first ATP competitive small molecule IGF-1R inhibitors reported with more than 10-fold selectivity over IR. However, despite the initial claimed selectivity window over IR for this series of compounds, some recent reports refer to compound 1a as a dual IGF-1R/IR inhibitor with equal potencies against both receptors.[22]

Figure 2.

Adenosine triphosphate competitive insulin-like growth factor 1 receptor inhibitors with reported selectivity over insulin receptor.

Another reported small molecule ATP competitive IGF-1R inhibitor with selectivity over IR is compound 2 (PQIP, Figure 2).[23] The cellular pIGF-1R (human) IC50 of PQIP was 19 nM as measured in 3T3/huIGF1R cells. This compound also showed a cellular pIR (human) IC50 of 261 nM in HepG2 cells and a cellular pIR (mouse) IC50 of 90 nM in Hepa-1 cells, thus an ~14-fold IGF-1R (human)/IR (human) selectivity was achieved based on comparison of IC50 values. However, a narrower window (~4-fold) was achieved when comparing potencies against IGF-1R (human) and IR (mouse). PQIP displayed potent anti-proliferative effects in a number of colorectal, breast, and pancreatic cancer cell lines, and further showed significant (>90%) TGI in multiple xenograft models including 3T3/huIGF1R and GEO (colorectal model) at an oral dose of 100 mg/kg.

In terms of non-ATP competitive IGF-1R inhibitors, cyclolignan picropodophyllin, a molecule of natural product origin (PPP, AXL1717, compound 3), was reported with potent cellular pIGF-1R activity (IC50=40 nM) without effects against pIR.[24] It also uniquely induced IGF-1R degradation, which was thought to contribute to its anti-tumor activity. In pre-clinical studies, 3 is efficacious in a variety of tumor models including those derived from breast, prostate, melanoma and multiple myeloma.[25-27] However, the mode of action of this compound has been called into question based on its microtubule inhibition activity and ability to induce cell death in IGF-IR–deficient cells.[28] AXL1717 has advanced into clinical trials (Table 2). Currently, in a phase II randomized, open-label study, the effectiveness and safety of AXL1717 is being compared to docetaxel in patients with previously treated, locally advanced, or metastatic squamous cell carcinoma or adenocarcinoma of the lung (NCT01561456). Additionally, AXL1717 is being evaluated in a phase I trial in combination with gemcitabine and carboplatin against previously untreated, locally advanced, or metastatic squamous non-small-cell lung cancer (NCT01466647).

Table 2.

PPP/AXLl717: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R inhibitor	Phase	Indication	Trial ID
	I	Advanced malignant tumors	NCT01725555
	I/II	Recurrent malignant astrocytomas	NCT01721577
	II	Previously treated, locally advanced, or metastatic squamous cell carcinoma or adenocarcinoma of the lung	NCT01561456

IGF-1R, insulin-like growth factor 1 receptor.

It should be noted that in such cases where cellular selectivity is reported for a respective IGF-1R inhibitor, it is unclear as to how this selectivity translates over to different cell lines as well as to the in vivo setting. The selectivity of IGF-1R over IR for an inhibitor might be further validated by studies that demonstrate that the selectivity is not just specific to a particular cell line and is, therefore, translatable across multiple cell lines and ideally into the in vivo setting. The availability of IGF-1R and IR dependent xenograft models offers the opportunity to determine whether the observed in vitro selectivity is transferable to the in vivo setting where PK/PD/Efficacy relationships can be established and linked to IGF-1R selectivity over IR.

Development of type I insulin-like growth factor receptor inhibitors based on compensatory signaling/pathway cross talks

In recent years, the biology around IGF-1R has continued to advance and has revealed that IGF-1R signaling engages cross-talk interactions with various feedback, compensatory and redundant signaling pathways in cancer cells. This phenomenon provides cancer cells with additional survival pathways when IGF-1R signaling is suppressed, and may help to explain the marginal clinical success achieved to date by agents that selectively target IGF-1R, through either mAbs or small molecules. The field has since migrated toward a multi-targeting strategy in order to achieve enhanced efficacy through either an additive or synergistic effect. This strategy can be realized by two approaches: i) combination of an IGF-1R inhibitor with other molecular targeted agents (multi-drugs multi-targets); or ii) design of specific multi-targeting activities [(i.e. IGF-1R and IR or IGF-1R and epidermal growth factor receptor (EGFR)] into a single molecule (single-drug multi-targets). Both approaches, in theory, can be empirically guided by established biological rationale; however, each is presented with unique challenges. When combining agents, the potential for drug-drug interactions must be considered. Along with enhanced efficacy, the potential is introduced for enhanced toxicities and subsequent reduced tolerability. In addition, the feasibility of combining more than two agents, which includes a tolerability as well as cost component, must be taken into consideration. The latter approach, the design of multi-targeted and ideally rationally designed selectively non-selective inhibitors remains a challenge for drug discoverers.[29] Achieving the right balance between building in preferred targets and building out dose-limiting off-targets to afford a truly selective multi-targeted inhibitor and not a highly promiscuous inhibitor remains a challenge due to the structural differences or lack thereof between targets within and outside a target class (e.g. kinases, G protein coupled receptors, ion channels). As various cross-talk interactions engaging IGF-1R have been reported,[30-32] this review will focus on interactions of IGF-1R with kinases of therapeutic significance in cancer, including IR, EGFR, the mammalian target of rapamycin (mTOR) and mitogen-activated protein kinase kinase (MEK). Additionally, the multi-drugs multi-target and single-drug multi-target approaches employed to target the IGF-1R cross-talk network will be discussed within.

Type I insulin-like growth factor receptor and insulin receptor signaling interactions

Pre-clinical research has demonstrated that IR signaling may also promote tumor growth and in this manner share redundancies with IGF-1R signaling. IR has been shown to promote tumor cell survival and proliferation both in vitro and in vivo.[33-36] Detailed studies further demonstrate that IR is able to drive cell growth upon activation by IGF-2 through autocrine/paracrine mechanisms.[37,38] While IR can be further classified into two isoforms (namely IR-A and IR-B), IR-A appears to be the primary contributor in cancer cell biology since this isoform is the predominant isoform of IR expressed in many tumor cells and is activated potently by both insulin and IGF-2.[39] Epidemiological data also support a role for IR in cancer, where elevated levels of insulin are a poor prognostic indicator for prostate and breast cancer patients. In addition, overexpression of IR has been observed in several types of cancers such as breast, ovarian, and thyroid.[40-42]

More recent studies have established that there is reciprocal cross talk between IR and IGF-1R. IR can form a heterodimer with IGF-1R, and this heterodimer can be activated by the growth factor ligands IGF-1, IGF-2 and insulin (Figure 3). In normal cells that co-express both IGF-1R and IR, IR activity may be up-regulated in a compensatory manner upon inhibition of IGF-1R. For example, disruption of IGF-1R in osteoblasts enhances insulin signaling and action,[43] and insulin-stimulated IRS-1 phosphorylation is elevated in IGF-1R knockout cells.[44] Recent studies have shown that cross-talk resonates between IGF-1R and IR in human tumor cells. For example, treatment with an IGF-1R specific antibody is associated with elevated signaling through IR, which may limit sustained inhibition of AKT signaling (Figure 4).[34] In contrast, the dual IGF-1R/IR inhibitor OSI-906 is capable of reducing phosphorylation of both receptors. In head-to-head studies comparing these two agents, OSI-906 displays superior efficacy compared to an IGF-1R specific antibody in human tumor xenograft models in which both IGF-1R and IR were phosphorylated (Figure 5).[34] Taken together, these data strongly suggest that co-targeting both IGF-1R and IR is critical to achieve superior and broader anti-tumor efficacy as compared to targeting IGF-1R alone.

Figure 3.

Insulin-like growth factor 1 receptor (IGF-1R)-insulin receptor (IR) reciprocal interactions: signal transduction from extracellular stimuli such as IGF-1, IGF-2 and insulin to intracellular pathways is mediated through IGF-1R, IR and IGF-1R/IR heterodimers. Furthermore, IR activity may be up-regulated in a compensatory manner upon inhibition of IGF-1R.

Figure 4.

Compensatory activation of pIR observed upon treatment with MAB-391 but not OSI-906 across multiple cancer cell lines.[34] NSCLC, non-small cell lung carcinoma; CRC, colorectal cancer; OvCa, ovarian carcinoma; EwS, Ewing’s sarcoma; ACC, adrenocortical carcinoma.

Figure 5.

(A) Tumor growth inhibition observed in GEO colorectal xenograft model with OSI-906 but not IGF-1R mAb, MAB392. (B) Compensatory activation of pIR and restoration of pAKT signaling observed following 24-h treatment with MAB-391 but not OSI-906.[34]

Recent developments in small molecule type I insulin-like growth factor receptor/insulin receptor dual inhibitors

The discovery and clarification of IGF-1R/IR compensatory signaling provided a rationale for co-targeting IGF-1R and IR. As a result, a variety of potent, bioavailable dual IGF-1R/IR inhibitors derived from more than 10 distinct chemotypes have been reported. Several review articles covering the historical developments of dual IGF-1R/IR inhibitors have been published in recent years, where the major chemotypes, as represented by compounds 4-13 in Figure 6 and Table 3, their potencies, and binding interactions have been summarized and discussed.[13-15] Here we will review and up-date the recent developments of the two most advanced clinical agents, OSI-906 (compound 4) and BMS-754807 (compound 6), as well as highlight very recent disclosures of pre-clinical compounds which have not been covered by previous reviews (compounds 14-15).

Figure 6.

Selected sdenosine triphosphate competitive dual insulin-like growth factor 1 receptor/insulin receptor inhibitors.

Table 3.

A summary of the current status of disclosed adenosine triphosphate competitive dual insulin-like growth factor 1 receptor/insulin receptor inhibitors.

Compound	Company	Current status
4 (OSI-906)	OSI	Phase-III
5 (FQIT)	OSI	Pre-clinical
6 (BMS-754807)	BMS	Phase II
7 (BMS-695735)	BMS	Pre-clinical
8 (BMS-536924)	BMS	Pre-clinical
9 (GSK1838705A)	GSK	Pre-clinical
10	GSK	Pre-clinical
11 (GSK1904529A)	GSK	Pre-clinical
12	Wyeth	Pre-clinical
13	Wyeth	Pre-clinical
14	Amgen	Pre-clinical
15	AZ	Pre-clinical

OSI-906

OSI-906 is a potent, dual IGF-1R/IR inhibitor derived from an imidazo[1,5-a]pyrazine scaffold. As shown in Figure 7, compound 16 represented an unoptimized early hit from the series with a benzyloxyphenyl moiety at the C1 position with moderate IGF-1R potency (cellular pIGF-1R IC50=1.2 M). Binding interaction optimizations driven by structure-based drug design (SBDD) with both IGF-1R and IR co-crystal structures led to the identification of a 2-phenylquinoline sub-series as exemplified by compound 17 which showed a significant improvement in potency (cellular pIGF-1R IC50=86 nM) but suboptimal drug metabolism and pharmacokinetic (DMPK) properties as a result of metabolism at the C3 position of the cyclobutyl ring. Further optimization of potency and DMPK properties led to more advanced compounds such as 18 (AQIP),[45] 2 (PQIP)[23] and eventually to the clinical agent, OSI-906 (linsitinib, compound 4).[46] OSI-906 potently inhibits IGF-1R and IR in the cellular setting. It demonstrates good oral bioavailability across multiple pre-clinical species as well as significant tumor growth inhibition in multiple tumor xenograft models, including NIH-3T3/LISN, GEO [colorectal cancer (CRC)], H295R [adrenocortical carcinoma (ACC)], and IGF-1R and IR direct complementary (DC) models.

Figure 7.

Evolution of dual insulin-like growth factor 1 receptor/insulin receptor inhibitors derived from an imidazo[1,5-a]pyrazine scaffold and structure-based drug design efforts.

Compared to other disclosed small molecule dual IGF-1R/IR inhibitors, OSI-906 has uniquely demonstrated exquisite selectivity when screened against a panel of 442 kinases (KinomeScanTM, DiscoveRx Corporation, Fremont, CA, USA), only inhibiting the IGF axis receptors; selectivity score (S-score) 0.008. The high degree of selectivity is attributed to unique binding interactions of OSI-906 with both IGF-1R and IR which stabilize both receptors in an intermediate conformation between active and inactive states.[46] OSI-906 completed dose-escalating phase I clinical trials in humans.[47,48] OSI-906 is orally bioavailable and noted to have an acceptable safety profile in humans. A maximum tolerated dose of 150 mg bid was achieved on a continuous dosing schedule where sustained plasma concentrations above the threshold required for anti-tumor efficacy in pre-clinical models were exceeded. Although hyperglycemia was evident in patients treated with OSI-906, a PK/PD relationship was observed where OSI-906 inhibited both p-IGF-1R and p-IR in peripheral blood mononuclear cells of cancer patients, with the degree of inhibition correlating with OSI-906 plasma levels. Encouraging disease control rate for response in evaluable patients was observed. One patient with ACC had a confirmed partial response at 16 weeks of treatment with OSI-906 and remained on the study for over 90 weeks with no drug-related toxicities observed. This response, in conjunction with pre-clinical efficacy in ACC xenograft models, led to the design of a randomized phase III study in ACC with OSI-906 as a single agent. Major emphasis for the ongoing clinical development plan is centered around combination therapy, and OSI-906 is being evaluated in multiple advanced clinical studies including combination with paclitaxel for the treatment of ovarian cancer and in combination with erlotinib for the treatment of NSCLC (Table 4).

Table 4.

OSI-906: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R inhibitor	In combination with	Phase	Indication	Trial ID
OSI-906	—	I	Advanced solid tumors	NCT01529684
	—	II	Relapsed small cell lung cancer	NCT01533181
	—	II	Asymptomatic or mildly symptomatic metastatic prostate cancer	NCT01533246
	—	II	Gastrointestinal stromal tumors	NCT01560260
	—	II	Relapsed small cell lung cancer	NCT01387386
	Irinotecan	I	Advanced cancer	NCT01016860
	Everolimus	I	Metastatic colorectal cancer	NCT01154335
	Paclitaxel	I/II	Recurrent epithelial ovarian cancer (and other solid tumors)	NCT00889382
	Erlotinib, radiation therapy	I/II	Advanced-stage cutaneous squamous cell carcinoma of the head and neck	NCT01465815
	Erlotinib	II	Advanced NSCLC with activating mutations in EGFR	NCT1221077
	Erlotinib	II	Maintenance therapy in patients with non-progression following chemotherapy in NSCLC	NCT01186861
	Cetuximab	II	Platinum-refractory, recurrent/metastatic head and neck squamous cell carcinoma	NCT0142720

IGF-1R, insulin-like growth factor 1 receptor; NSCLC, non-small cell lung carcinoma; EGFR, epidermal growth factor receptor.

BMS-754807

BMS-754807 (compound 6) is a pyrrolotriazine-based IGF-1R inhibitor which evolved from an earlier pyrazolopyrimidine series (e.g. compound 19) through medicinal chemistry optimization (Figure 8).[49] This molecule inhibited both IGF-1R and IR with equal potency (enzyme biochemical IC50=1.7 nM (IGF-1R); 1.8 nM (IR), measured at [ATP]=Km for each kinase). It also inhibited the phosphorylation of IGF-1R potently in the IGF-Sal cell line with an IC50 of 13 nM. This compound showed potent in vitro anti-proliferative effects and demonstrated significant TGI effects in multiple human tumor xenograft models when dosed orally. BMS-754807, a type I kinase inhibitor, has been reported to have off-target activities against other kinases, some of which have been implicated in cancer growth and survival. It is not clear as to whether these off-target activities are significantly inhibited in humans and offer a benefit or present dose limiting toxicities. BMS-754807 is currently in multiple advanced clinical trials, including a phase II study against hormone receptor-positive breast cancer (resistance to non-steroidal aromatase inhibitors), as well as in advanced or metastatic solid tumors (colorectal cancer, head and neck cancer, neoplasm metastasis) as a single agent in combination with cetuximab (Table 5). BMS-754807 was also evaluated in combination with trastuzumab against advanced or metastatic Her-2-positive breast cancer (NCT00788333, completed, data not disclosed to date), and in combination with paclitaxel and carboplatin against advanced or metastatic solid tumors (NCT00793897, completed, data not disclosed to date).

Figure 8.

Pyrrolotriazine-based dual insulin-like growth factor 1 receptor/insulin receptor inhibitors 6 (BMS-754807) evolved from pyrazolopyrimidine scaffold.

Table 5.

BMS-754807: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R inhibitor	In combination with	Phase	Indication	Trial ID
BMS-754807	—	I	Advanced or metastatic solid tumors	NCT00569036
	Cetuximab	I/II	Advanced or metastatic solid tumors	NCT00908024
	Letrozole	II	Hormone receptor-positive breast cancer	NCT01225172

IGF-1R, insulin-like growth factor 1 receptor.

Most recent preclinical disclosure of type I insulin-like growth factor receptor/insulin receptor inhibitors

In 2011, a series of 2,4-bis-arylamino-1,3-pyrimidines were disclosed by Amgen as dual IGF-1R and IR inhibitors.[50] As shown in Figure 9, medicinal chemistry efforts initiated from triazine-derived screening hit 20 (cellular pIGF-1R IC50=175 nM). Progression to a pyrimidine core afforded compound 21 and a nearly 10-fold potency improvement (cellular pIGF-1R IC50=19 nM) as a result of increased binding interactions and a decrease in the desolvation energy from the binding process. Further analoging around the aniline pharmacophore led to the identification of 14 with a cellular pIGF-1R IC50 value of 81 nM, ~4-fold less potent than that of 21. Both compounds 14 and 21 were further assessed in vivo in a Calu-6 tumor xenograft model. Interestingly, the less potent analog 14 demonstrated tumor growth inhibition of 56% at an oral dose of 100 mg/kg bid, while the more potent analog 21 failed to show any efficacy (0% TGI) at the same dose and dosing regimen. The authors attributed the efficacy of 14 to the achievement of high levels of tumor drug concentrations. In a single dose mouse PK study, compound 14 displayed a large volume of distribution (Vss) of 28 L/kg that translated into very high tumor drug concentrations (Cmax=142.9 M at 100 mg/kg dose) despite a much lower plasma drug exposure (Cmax=2.2 M at 100 mg/kg dose). In contrast, compound 21 displayed a lower Vss of 0.3 L/kg, which in turn resulted in lower tumor drug concentrations (Cmax=2.7 M at 100 mg/kg dose) although it showed a higher plasma drug exposure (Cmax=13.4 M at 100 mg/kg dose). Strong PD inhibition (~80%) of pIGF-1R was observed for compound 14 from the aforementioned xenograft study at the 100 mg/kg dose, but not at 30 mg/kg which may be the result of significantly lower tumor drug concentrations (Cmax=1.36 M). Compound 14 was selective against cell cycle regulators Aurora A, CDK2 and several kinases involved in tumor cell growth and differentiation, including MET, EGFR, FGFR, KDR and Tie2. Selectivity of this compound against a larger panel of kinases has not been disclosed.

Figure 9.

Optimization of 2,4-bis-arylamino-1,3-pyrimidines based dual insulin-like growth factor 1 receptor/insulin receptor (IGF-1R/IR) inhibitors led to compound 14. The proposed binding mode and major hydrogen bond interactions of 14 with IGF-1R based on a co-crystal structure of a related analog (PDB code: 3QQU).

In early 2012, AstraZeneca reported on an imidazo[1,2-a]pyridine series of IGF-1R/IR inhibitors.[51,52] As shown in Figure 10, compound 22, which emerged from a historical CDK2 program, was identified from an IGF-1R cell-based HTS campaign as a moderate IGF-1R inhibitor. The CDK2 activity was successfully dialed out with the retention of IGF-1R activity as a result of modifications to the aniline pharmacophore (compound 23). Substitutions on the pyrimidine moiety especially with halogens significantly increased potency. For example, in the case where a bromine atom was implemented (compound 25), a remarkable ~150-fold improvement was achieved in both biochemical and cellular potencies when compared to the non-substituted analog 23. Further medicinal chemistry analoging efforts on the imidazopyridine pharmacophore did not yield any additional improvements. Compound 15 was selected for further profiling and was shown to be orally bioavailable in multiple pre-clinical species including mouse, rat and dog (F%>30%); however, no in vivo efficacy data has been disclosed. The kinase selectivity of 15 was evaluated in a panel of 69 kinases at a compound concentration of 1 M, with 3 kinases, JNK1 (MAPK8), JNK2 (MAPK9) and ERK8 (MAPK15) being inhibited at over 80%.

Figure 10.

Optimization of imidazo[1,2-a]pyridine-based dual insulin-like growth factor 1 receptor (IGF-1R) and insulin receptor (IR) inhibitors.

Type I insulin-like growth factor receptor and epidermal growth factor receptor signaling interactions

Although both small molecule and antibody EGFR inhibitors have demonstrated clinical utility,[53] resistance often develops in the clinic following longer term treatment. In pre-clinical models, interaction between IGF-1R and EGFR signaling has been shown to be a contributing mechanism to resistance to anti-EGFR therapies (Figure 11). For example, in early stage NSCLC patients, IGF-1R protein expression was shown to be associated with EGFR protein expression and elevated coexpression of both IGF-1R and EGFR correlates with poor prognosis, as evidenced by shorter disease-free survival.[54] Reciprocal interaction between IGF-1R and EGFR has also been described in a variety of other tumor types, including breast cancer, CRC, pancreatic cancer (PaCa) and HCC, where inhibition of either receptor can promote the activation of the other receptor.[55-58] Multiple mechanisms for IGF-1R/EGFR interaction have been proposed, including direct association and activation between the two receptors, modulation of the availability of reciprocal ligands, or through interactions with common partners or downstream effectors.[59]

Figure 11.

Reciprocal interaction between insulin-like growth factor 1 receptor (IGF-1R) and epidermal growth factor receptor (EGFR) where inhibition of either receptor can promote the activation of the other receptor.

In pre-clinical studies, co-targeting EGFR and IGF-1R was shown to produce superior efficacy compared to treatment with the respective monotherapies in multiple models.[60,61] For example, the combination of erlotinib and an IGF-1R TKI, such as PQIP or OSI-906, leads to a synergistic increase in apoptosis in multiple cell lines including H292 (Figure 12) as well as synergistic tumor growth inhibition, regressions and enhanced cure rates in xenograft models of NSCLC and pancreatic cancer (Figure 13).[62] Collectively, these pre-clinical studies strongly support the hypothesis of co-targeting IGF-1R and EGFR signaling as a novel approach to achieve superior clinical response and prevent/minimize drug resistance due to IGF-1R/EGFR reciprocal cross talk. This hypothesis is currently being evaluated in multiple clinical trials (multi-drug multi-target approach) as highlighted in Table 6.

Figure 12.

Synergistic increase in apoptosis observed in vitro with the combination of insulin-like growth factor 1 receptor (IGF-1R)/insulin receptor dual inhibitor OSI-906 and epidermal growth factor receptor inhibitor erlotinib (10 uM). Either erlotinib or OSI-906 alone had minimal (<2-fold) effect on caspase 3/7 activity; however, the combination results in more than 12-fold increased caspase 3/7 activity (E. Buck, M.J. Mulvihill, et al., 2013, unpublished results).

Figure 13.

Enhanced tumor growth inhibition observed with the combination of insulin-like growth factor 1 receptor/insulin receptor dual inhibitor OSI-906 and epidermal growth factor receptor inhibitor erlotinib E. Buck, M.J. Mulvihill, et al., 2013, unpublished results).

Table 6.

Insulin-like growth factor 1 receptor inhibitor in combination with epidermal growth factor receptor/HER2 inhibitor: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R inhibitor	In combination with EGFR or HER2 inhibitor	Phase	Indication	Trial ID
AMG479	Panitumumab	II	Wt K-Ras metastatic colorectal cancer	NCT00891930
	Panitumumab	II	Colorectal cancer	NCT00788957
IMC-A12 (Cixutumumab)	Cetuximab	II	Head and neck squamous cell carcinoma	NCT00957853
OSI-906	Cetuximab	II	Platinum-refractory, recurrent/metastatic head and neck squamous cell carcinoma	NCT01427205
	Erlotinib	I/II	Advanced-stage cutaneous squamous cell carcinoma of the head and neck	NCT01465815
	Erlotinib	II	Advanced NSCLC with EGFR activating mutations	NCT01221077
	Erlotinib	II	Maintenance therapy in patients with non-progression following chemotherapy in NSCLC	NCT01186861
BMS-754807	Cetuximab	I/II	Advanced or metastatic solid tumors	NCT00908024

IGF-1R, insulin-like growth factor 1 receptor; EGFR, epidermal growth factor receptor; NSCLC, non-small cell lung carcinoma.

Recent developments in small molecule inhibitors co-targeting both type I insulin-like growth factor receptor and epidermal growth factor receptor

The strong rationale previously described for co-targeting IGF-1R/IR and EGFR through the combination of selective inhibitor provided the scientific basis to pursue a single molecule that could selectively target both pathways. Developments in this area utilizing the single-drug multi-target approach has been reported by Abbott Laboratories around a series of imidazo[2,1-b]thiazole and pyrazolo[3,4-d]pyrimidine derived IGF-1R inhibitors (Table 7).[63-65] The imidazo[2,1-b]thiazole series, as highlighted by compound 26, displayed significant potency versus IGF-1R in A431cells with an IC50 value of 41 nM and modest EGFR and ErbB2 potencies of 350 and 310 nM, respectively. From the pyrazolopyrimidine class, compound 27a was reported to inhibit all three targets with a cellular IC50 of ~100 nM. Unfortunately, the overall kinase selectivity profile of this compound was not reported and, therefore, these cellular activities are unable to be placed into a proper context. Compound 27a displayed moderate mouse PK properties (oral bioavailability 12%) and demonstrated significant PD inhibition of both pIGF-1R and pEGFR in a mouse model. Unfortunately, no in vivo efficacy or tolerability results were reported. From the same pyrazolopyrimidine chemotype, compound 27b was highlighted as an advanced analog, displaying cellular potencies (IC50 values) versus IGF-1R, pEGFR and pErbB2, of 207, 2300 and 340 nM, respectively. The oral bioavailability was modest, at 20% in the mouse. Compound 27 was evaluated in an in vivo PD model where intravenous dosing at 30 mg/kg demonstrated 50% inhibition of pIGF-1R; however, PD versus EGFR or ErbB2 was not reported. The kinase selectivity of compound 27 was assessed against 80 kinases and the results showed potent inhibition of several other kinases including the Aurora family. No in vivo tumor growth inhibition data were reported. Collectively, these efforts highlight the challenges as noted by Morphy[29] associated with achieving highly selective nonselective kinase inhibitors, when targeting structurally distinct kinase family members.

Table 7.

Enzyme and cellular IC50 values for select pyrazolo[3,4-d]pyrimidine and imidazo[2,1-b]thiazole-derived insulin-like growth factor 1 receptor/epidermal growth factor receptor/ErbB-2 inhibitors.

Compound	Enzyme (cellular) IC50 nM
	IGF-1R	EGFR2*	Erb-B2
26°	52 (41)	16 (350)	170 (310)
27a#	81 (115)	58 (85)	54 (94)
27b§	12.5 (207)	31.5 (2300)	7.5 (340)

IGF-1R, insulin-like growth factor 1 receptor; EGFR, epidermal growth factor receptor.

*EGFR construct with L858R mutation;

°ELISA assays of receptor auto-phosphorylation, in A431cells for pIGF-1R and pEGFR and N87 cells for pErbB2;

#ELISA assays of receptor auto-phosphorylation, in MiaPaCa cells for pIGF-1R and pEGFR and N87 cells for pErbB2;

§ELISA assays of receptor auto-phosphorylation, in MiaPaCa cells for pIGF-1R and pEGFR and BT474 cells for pErbB2.

Ranbaxy Laboratories recently disclosed compound 28 as a dual IGF-1R/EGFR inhibitor derived from a bis-arylamino-pyrimidine scaffold.[66] This compound has balanced and potent IGF-1R and EGFR activities, and showed superior anti-proliferative effects in multiple cell lines, such as A431, HT29, and A549, when compared to EGFR inhibitor erlotinib alone or IGF-1R inhibitor NVP-AEW541 (compound 1a) alone (Table 8). Compound 28 also showed anti-proliferative sensitivity in H1975 cells with a GI50 of 1.3 M, a cell line that harbors an EGFR mutation (T790M) and reported to be resistant to erlotinib (GI50 of 47 M). The authors attributed the observed efficacy to the unique multi-targeted profile of compound 28, although it is not clear if compound 28 directly inhibits EGFR with the T790M mutation. The kinase selectivity of this compound was evaluated in a focused kinase panel at a concentration of 10 M, where no significant inhibition (<50%) of kinases such as FGFR, Aurora A, GK, Wee-1 and Erk-1, was observed. Interestingly, only moderate inhibition of ErbB-2 (55% inhibition) was observed at this concentration, providing a potential point of differentiation to IGF-1R/EGFR/ErbB-2 inhibitors 26 and 27. Unfortunately, poor mouse PK properties associated with this compound as indicated by high plasma clearance and low T1/2 prevented it from being further evaluated in animal studies (e.g. mouse xenograft efficacy and tolerability studies).

Table 8.

Small molecule inhibitor co-targeting insulin-like growth factor 1 receptor and epidermal growth factor receptor.

Compound	Enzymatic IC50 (nM)		Anti-proliferative IC50 (nM)
	IGF-1R	EGFR	A431	HT29	A549
Erlotinib	>10,000	45	1080	2275	>10,000
28	74	45	170	274	111
1a	291	>10,000	899	9540	615

IGF-1R, insulin-like growth factor 1 receptor; EGFR, epidermal growth factor receptor.

Within the field of dual IGF-1R/EGFR inhibitors, what appears to be lacking is a head-to-head in vivo comparison of selective dual IGF-1R/EGFR inhibitors to selective compounds only targeting IGF-1R and/or EGFR in respect to both efficacy and tolerability. Furthermore, it would be of interest to determine if such specifically designed multitargeted inhibitors display a superior or differentiated profile (e.g. efficacy, tolerability) to that of the combination of a selective IGF-1R/IR inhibitor with a selective EGFR/Erb2 inhibitor. Unfortunately, no such comparative data have been disclosed to date.

Type I insulin-like growth factor receptor and mammalian target of rapamycin signaling interactions

Studies of the PI3K/AKT/mTOR pathway have revealed that inhibition of mTORC1 by a rapamycin analog led to upregulation of AKT activity via the S6K-IRS2 negative feedback loop and thus rendering the mTORC1 inhibitor less effective.[67] Since inhibition of IGF-1R leads to downregulation of AKT signaling, it was then hypothesized that inhibiting both mTORC1 and IGF-1R may counteract this feedback loop and produce a superior therapeutic response compared to mTORC1 inhibition alone. This hypothesis has been confirmed in pre-clinical studies by using a combination of rapamycin and the IGF-1R inhibitor NVP-AEW541 (compound 1a).[67] A recent study assessing the combination of ridaforolimus (MK-8669, mTORC1 inhibitor) and dalotuzumab (MK-0646, IGF-1R mAb) also showed similar results.[68] In this study, a panel of over 60 breast cancer cell lines were screened with ridaforolimus to test this hypothesis. It was found that ridaforolimus treatment up-regulated multiple key nodes of the IGF-1R pathway and provided the rationale for the mTORC1/IGF-1R combination. Eventually, Lum-B breast cancer was determined to be the most suitable for this combination study due to its ER+ characteristic (correlates with sensitivity of ridaforolimus) and highest IGF-1R mRNA level. Based on encouraging pre-clinical results, the combination of ridaforolimus and dalotuzumab is currently being evaluated in multiple phase I and phase II trials (Table 9). Based on similar biological rationale, R1507, an IGF-1R mAb is also being evaluated in a phase I study in combination with mTORC1 inhibitor everolimus.

Table 9.

Insulin-like growth factor 1 receptor inhibitor in combination with mTORC1 inhibitors: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R inhibitor	In combination with mTORC1 inhibitor	Phase	Indication	Trial ID
R1507	Everolimus	I	Advanced solid tumors	NCT00985374
AMG479 (Ganitumab)	Everolimus	I	Advanced solid tumors	NCT01122199
IMC-A12 (Cixutumumab)	Everolimus	I	Neuroendocrine carcinoma	NCT01204476
	Temsirolimus	I/II	Metastatic prostate cancer	NCT01026623
	Temsirolimus	I/II	Locally recurrent or metastatic breast cancer	NCT00699491
	Temsirolimus	II	Advanced cancers	NCT00678769
	Temsirolimus	II	Metastatic sarcomas	NCT01016015
	Temsirolimus	II	Pediatric patients with recurrent or refractory solid tumors	NCT01614795
MK-0646 (Dalotuzumab)	Ridaforolimus	I	Advanced cancers	NCT01243762
	Ridaforolimus	I	Advanced solid tumors	NCT01431547
	Ridaforolimus	II	Estrogen receptor positive breast cancer	NCT01234857
OSI-906	Everolimus	I	Metastatic colorectal cancer	NCT01154335

IGF-1R, insulin-like growth factor 1 receptor.

It has recently been shown that the tumor suppressor gene, LKB1 is lost in ~35% of NSCLC. LKB1 plays a critical role in energy sensing and regulates the PI3K/mTOR pathway.[69] Loss of LKB1 leads to activation of the mTOR and IGF-1R pathways.[70] Dual inhibition of IGF-1R and mTOR with dual IGF-1R/IR TKI OSI-906 and dual mTORC1/2 inhibitor OSI-027[71] synergistically inhibits proliferation in several pre-clinical models with LKB1 loss (mutation) including H1437, A427, H2126 and H1395. The combination of IGF-IR + mTOR inhibition with OSI-906 and OSI-027 was more effective than either monotherapy in the H1437 mouse xenograft model.[70]

Type I insulin-like growth factor receptor and mitogen-activated protein kinases signaling interactions

IGF-1R signaling has also been implicated in drug resistance developed following treatment with a myriad of other anti-tumor agents including inhibitors acting within the MAPK pathway. Treatment with an MEK kinase inhibitor has been shown to result in elevated IGF-driven AKT signaling, and the combination of the dual IGF-1R/IR inhibitor OSI-906 with an MEK inhibitor has been shown to inhibit tumor cell proliferation in a synergistic manner.[62] Furthermore, MEK inhibitors in combination with an IGF-1R inhibitor (AXL1717) induce cell death in tumor cells with acquired resistance to a RAF inhibitor.[72] There is also clinical data highlighting the potential for IGF-1R to play a role in resistance to MAPK pathway inhibitors. For example, resistance following long-term treatment with the B-RAF inhibitor vemurafenib in melanoma patients is associated with elevated IGF-1R expression.[73] These data suggest a combination of a MAPK pathway inhibitor and an IGF-1R inhibitor may overcome certain clinically observed drug resistance to vemurafenib. Currently, IGF-1R monoclonal antibody AMG479 is being evaluated in a clinical trial in combination with MEK1/2 inhibitor MEK162 against advanced solid tumors (Table 10).

Table 10.

Insulin-like growth factor 1 receptor inhibitor in combination with mitogen-activated protein kinases pathway inhibitor: ongoing clinical trials as of January 2013 (www.clinicaltrials.gov).

IGF-1R inhibitor	MAPK pathway inhibitor	Phase	Indication	Trial ID
AMG479 (Ganitumab)	MEK162	lb/II	Selected advanced solid tumors	NCT01562899

IGF-1R, insulin-like growth factor 1 receptor; MAPK, mitogen-activated protein kinases.

Promiscuous kinase inhibitors with significant type I insulin-like growth factor receptor activities

XL228 is a multikinase inhibitor with potent activities against IGF-1R, SRC family kinases, BCR-ABL, FGFR1-3 (fibroblast growth factor receptors 1-3) and the aurora kinases. This compound was derived from a 2,4-disubstituted pyrimidine series although detailed information about its structure has not been disclosed. XL228 was progressed into two phase I clinical trials (NCT00464113, NCT00526838) and early clinical data showed evidence of IGF-1R and SRC kinase pathway inhibition, as supported by phospho-protein analysis in circulating leukocytes, hair follicles and skin biopsy samples, and by transient upregulation of plasma glucose and insulin. It was generally well tolerated at its maximum tolerated dose of 6.5 mg/kg, and showed evidence of single agent anti-tumor activity which included a confirmed partial response in a NSCLC patients.[74] However, both trials have been terminated and no new clinical activity of this compound has been disclosed to date.

A class of catechol derivatives was reported as IGF-1R inhibitors, most likely operating through a non-ATP competitive manner. Some representative compounds are shown in Figure 14. From this class, natural product 30 (NDGA, INSM-18)[75] has progressed into phase-I/II clinical trials against non-metastatic hormone-sensitive prostate cancer. Compound 30 was dosed at 2000 mg/day orally without any reported significant toxicities. However, it was recently reported that analysis showed no significant decline in prostate-specific antigen after three cycles of treatment among the first 12 patients enrolled.[76] It should be pointed out that compound 30 also has activities against lipoxygenase and other kinases such as ErbB-2 and FGFR3.[77] Both compounds 31 and 32 are synthetic analogs with only moderate IGF-1R potencies and remain to date in the pre-clinical stage. There are additional small molecule IGF-1R inhibitors that have been reported to have progressed into clinical trials, such as KW2450 (NCT00921336, NCT01199367) and PL2258 (NCT01779336). While these are certainly interesting developments, it is difficult to make any further comments on these agents since no information as to the structure or any pharmacological details of these compounds have been disclosed.

Figure 14.

Catechol derivatives as non-adenosine triphosphate competitive insulin-like growth factor 1 receptor inhibitors.

Conclusions

Since the initial discovery of the involvement of IGF-1R signaling in human cancer in the 1980s,[1-3] pre-clinical studies have provided a foundation for targeting IGF-1R signaling as a potential treatment for cancer. Consequently, numerous approaches have been undertaken to modulate IGF-1R activity, resulting in the progression of multiple agents into human clinical trials for the ultimate validation of IGF-1R as a cancer target. The plethora of drug discovery efforts around IGF-1R was pioneered by monoclonal antibodies which specifically target the ligand binding extracellular domain of this receptor,[78] and this was then followed by small molecule IGF-1R kinase inhibitors with both ATP competitive and non-ATP competitive binding modes. Unlike monoclonal antibodies that are highly specific for the designated target, small molecule kinase inhibitors can be tuned to include additional therapeutically beneficial off-target activities. The understanding of cancer biology around IGF-1R, and especially its role in various stages of cancer and its interactions with other signaling pathways, clearly influenced the design of small molecule IGF-1R kinase inhibitors. Historically, selective IGF-1R inhibitors that did not inhibit IR were pursued, due to concerns about potential toxicity that were suggested to arise from the inhibition of IR. Thus, initial efforts focused around creating selective IGF-1R agents and, therefore, avoiding IR inhibition through various strategies such as targeting allosteric binding sites. Although compounds with various degrees of selectivity (IGF-1R vs IR) have been reported and agents from this class have since progressed into clinical trials, success from this approach as single agents appears to be limited.

Recent research on IGF-1R signaling has focused on compensatory signaling as a resistance mechanism utilized by cancer cells for survival when IGF-1R activity is inhibited. Researchers now realize that resistance mechanisms involve a dynamic network of multiple intertwining signaling pathways. This includes interactions of IGF-1R with other kinases such as IR, EGFR, mTOR and MEK, as well as other receptors, such as the estrogen receptor.[79] These studies have suggested various possibilities of multi-drug multi-target and/or single-drug multi-target approaches to simultaneously block IGF-1R/IR signaling and other compensatory survival mechanisms as cancer treatments. Generally speaking, the multi-drugs multi-target approach can be successful when the combination of drugs are tolerated and provide greater efficacy. The risks and challenges associated with this approach are potential drug-drug interactions, complications in designing dose schedules and overall complications in drug combination clinical trial design. Nonetheless, drug combinations have become a common approach in clinical development, with examples in the oncology kinase field including the ongoing clinical evaluation of drug combinations co-targeting IGF-1R and EGFR, as well as MEK and EGFR, just to name a few.

Compared to the multi-drugs multi-target approach, the single-drug multi-target approach has the advantage of no risks related to drug-drug interactions and simplifies clinical trial design. This approach is particularly attractive when targeting multiple proteins that share relatively conserved binding sites, such as the ATP binding pocket of kinases. Kinases are also an example of a preferred target class for this approach because binding interactions are relatively well understood within ATP pockets and selectivity optimization can be greatly facilitated by taking advantage of available structural information via SBDD. The major challenge associated with this single-drug multi-target approach is engineering a molecule that possesses an optimal potency and selectivity profile against multiple targets. The compound optimization process could become a daunting task based upon the targets of interest when steering through multiple undesired off-targets while maintaining desired drug-like properties. Nonetheless, it is encouraging to see drug discovery efforts that have adopted the single-drug multi-target concept in recent years.[29,80,81] This approach has also been pursued in the IGF-1R field, as exemplified by small molecule dual IGF-1R/IR inhibitors and IGF-1R/EGFR inhibitors reviewed within. There is excitement in the oncology community around the multiple approaches and various drug combinations that are being actively pursued in the clinical setting based upon compelling and supporting pre-clinical data. It is our hope that ongoing clinical trials centered around IGF-1R will provide proof-of-concept for this target in humans and beneficial therapies for cancer patients around the world.