TY - JOUR
T1 - Liposomal Grb2 antisense oligodeoxynucleotide (BP1001) in patients with refractory or relapsed haematological malignancies
T2 - a single-centre, open-label, dose-escalation, phase 1/1b trial
AU - Ohanian, Maro
AU - Tari Ashizawa, Ana
AU - Garcia-Manero, Guillermo
AU - Pemmaraju, Naveen
AU - Kadia, Tapan
AU - Jabbour, Elias
AU - Ravandi, Farhad
AU - Borthakur, Gautam
AU - Andreeff, Michael
AU - Konopleva, Marina
AU - Lim, Miranda
AU - Pierce, Sherry
AU - O'Brien, Susan
AU - Alvarado, Yesid
AU - Verstovsek, Srdan
AU - Wierda, William
AU - Kantarjian, Hagop
AU - Cortes, Jorge
N1 - Funding Information:
In this phase 1/1b study of BP1001, an inhibitor targeted against GRB2, the drug was well tolerated both as monotherapy and in combination with low-dose cytarabine. We did not identify a maximum tolerated dose. The most common grade 3–4 adverse events were cardiopulmonary disorders, and fever (including neutropenic fever) and infections. BP1001 showed potential anti-leukaemic effects: nine (33%) of 27 patients in monotherapy cohorts had at least a 50% reduction in peripheral blood blasts, three (10%) of 29 patients in monotherapy cohorts had at least a 50% reduction in bone marrow blasts, and seven (22%) patients benefited from monotherapy (as per investigator's assessment) and had extended cycles of treatment. Furthermore, three (50%) of six assessable patients receiving BP1001 plus low-dose cytarabine combination therapy achieved complete recovery or incomplete haematological recovery. These data suggest that BP1001 has early evidence of anti-leukaemic activity in combination with low-dose cytarabine. We postulate that inhibition of Grb2 could curtail the progression of haematological malignancies because Grb2 is essential to the signalling of BCR-ABL, KIT, FLT3, and JAK2 tyrosine kinases, which are overexpressed or mutated in several leukaemias. 5–7 We selected an antisense strategy to inhibit Grb2 because Grb2 is an intracellular protein with no enzymatic activity. To target the GRB2 transcript, we used P-ethoxy antisense oligodeoxynucleotides, which do not contain locked nucleic acids or sulphur groups. Phosphorothioate antisense oligodeoxynucleotide, 19,20 gapmer antisense oligonucleotide containing locked nucleic acids, 21 2′-O-methoxy ethyl, 22 constrained ethyl residues, 23 and 2′-O-methyl RNA-containing mixed backbone antisense oligoucleotide 24,25 have been associated with complement activation, 19 coagulation, 19,20 and increased concentrations of serum transaminases 19,21–25 in oncology clinical trials. The Grb2 P-ethoxy antisense oligodeoxynucleotide was incorporated in the neutral DOPC lipid to enhance its biodistribution and intracellular uptake. 15 When complexed with negatively charged antisense oligodeoxynucleotides, cationic lipids could deposit aggregates in lung capillaries and cause an embolism. 26 Results from preclinical studies 15,16 showed that BP1001, administered at 15 mg/kg dose (equivalent to 45 mg/m 2 in human beings), extended the survival of mice bearing leukaemia xenografts without inducing excessive toxicity. The US Food and Drug Administration recommended the starting dose of BP1001 as a tenth of the efficacy dose used in this mouse survival study. 15,16 Thus, we used 5 mg/m 2 as the starting dose of BP1001 in phase 1. BP1001 was well tolerated. A maximum tolerated dose was not reached, even when BP1001 was administered at doses of 90 mg/m 2 . Contrary to many antisense oligodeoxynucleotides, 19,21–25 BP1001 did not induce an increase in serum transaminase concentrations. This finding might be due do the fact that BP1001 is packaged in a neutral liposome, made of naturally occurring DOPC lipids, and the P-ethoxy structure of the drug does not induce ribonuclease H activity, which has been linked with the hepatotoxicity of some antisense oligodeoxynucleotides. 27 However, this possibility remains to be tested. Thrombocytopenia 19,20,23,25 and prolongation of activated partial thrombin time (aPTT) 19,22,24 have also been reported for some antisense analogues, sometimes as dose-limiting toxicity. 21,23,24 Three patients in our study had grade 3–4 thrombocytopenia, but this was probably disease related since thrombocytopenia is common in this setting and was present at baseline. BP1001 did not seem to affect thrombocytopenia or aPTT. The two patients who had prolonged aPTT were given the lowest BP1001 dose, and aPTT was not observed in patients given higher BP1001 doses. These findings show that BP1001, which is composed of P-ethoxy oligodeoxynucleotide, has a very different toxicity profile to other antisense oligodeoxynucleotide analogues, which have been associated with thrombocytopenia, 19,20,23,25 aPTT prolongation, 22,24 and neurotoxicity. 28,29 Grb2 is upstream of pERK. A concomitant decrease in Grb2 and pERK concentrations was observed in 58% of assessed samples. However, there were a few instances in which a Grb2 decrease was not associated with pERK decrease, suggesting that in some instances, Grb2 might not be operating through pERK, or that other pathways in addition to Grb2 were activating pERK, but this warrants further investigation. Additionally, BP1001 did not reduce Grb2 concentrations in two patients. We speculate that this finding could have been possibly due to insufficient plasma concentrations of BP1001. Seven patients benefited from BP1001 monotherapy and had extended cycles of treatment while receiving monotherapy. These patients, who were refractory to at least one previous therapy regimen and no more than one previous salvage regimen, had diverse cytogenetic backgrounds: BCR–ABL, diploid, or complex mutations. Two patients had the JAK2 -V617F mutation, and two patients had the NRAS mutation. Increased Grb2 binding to the JAK2 -V617F mutant is expected because of the enhanced tyrosine kinase activity and phosphorylation of mutant JAK2 . 6 Since Grb2 is upstream of RAS, BP1001 benefiting patients with an NRAS mutation would not be expected. The three RAS family members have different post-translational modifications and subcellular localisations, resulting in consequent differential signaling. 30 NRAS signals through Raf and RhoA to regulate cell adhesion, whereas KRAS signals through Akt and Cell division control protein 42 (Cdc42) to regulate motility. 31 The function of NRAS is not clear, but paradoxically, patients with acute myeloid leukaemia with the NRAS mutation have been reported to have increased cytarabine sensitivity. 32 Patients with NRAS mutation might experience clinical benefit from BP1001 plus low-dose cytarabine. Further preclinical studies are evidently required in these subsets of patients to understand any possible role and the mechanism of action BP1001 might have in such instances. In this study, the highest tested dose of BP1001 was 90 mg/m 2 . BP1001 seemed to be cleared more rapidly at the 90 mg/m 2 dose than at the 60 mg/m 2 dose, decreasing its Vz and t 1/2 . It seemed that the uptake of BP1001 might have plateaued at 60 mg/m 2 , limiting BP1001 absorption even when a higher drug dose was administered. Preclinical and clinical reports show that liposomes are primarily taken up by mononuclear phagocytic cells of the liver, followed by those of the spleen, lungs, and bone marrow. 33 When liver uptake of liposomes is saturated, the excess liposomes are taken up by the spleen, leading to enhancement of liposome uptake. 26,33 This activity could result in a higher CL and shorter t 1/2 at higher BP1001 doses, although this has not been directly tested. A similar phenomenon has been observed with liposomal amphotericin B administered at 2·5 mg/kg compared with 1·0 mg/kg. 34 Our data indicate that Grb2 downregulation and potential anti-leukaemic effect in combination with low-dose cytarabine could be attained in participants at both doses, and safety and tolerability were not substantially different. Therefore, BP1001 is being administered at 60 mg/m 2 in combination with low-dose cytarabine in our ongoing phase 2 study. One of the limitations of this study was that the pharmacokinetic analysis was not reported for patients receiving BP1001 monotherapy. This was because of technical issues relating to the development of the sandwich ELISA to quantify Grb2 antisense oligodeoxynucleotide concentration in plasma and urine took some time to resolve, and prevented us from measuring these concentrations from the start of the study. When we tried to analyse the plasma and urine concentrations of BP1001 from patients in cohorts 1–6, the samples had been stored too long and were beyond their storage stability. Although we only report BP1001 samples from patients in the BP1001 plus low-dose cytarabine cohorts, samples were taken from patients on cycle one, day 1, before low-dose cytarabine was administered. We felt that the pharmacokinetic values of these samples reflected those of BP1001 monotherapy. We have recently acquired preliminary data suggesting that low-dose cytarabine might not interfere with our BP1001 ELISA, but this remains to be validated. Another limitation of the study is that we cannot formally state that we have identified the optimal biologically active dose. On day 15, the Grb2 and pERK downregulation effects appeared grossly similar between the 60 and 90 mg/m 2 BP1001 doses. At the end of treatment, a similar effect appeared to be reached with the 20, 60, and 90 mg/m 2 BP1001 dose range, because a 44–46% decrease in Grb2 concentrations was observed between these doses. We interpreted these results to suggest that further dose escalation was unwarranted as it appeared that we had reached a plateau in biological activity. Also, it would have been ideal to determine whether BP1001 could have a potential effect on leukaemia stem cells by determining whether BP1001 decreased Grb2 and pERK concentrations in the CD34-positive–CD38-negative cell population. To our knowledge, this is the first phase 1 study of a liposome-incorporated P-ethoxy antisense oligodeoxynucleotide targeted against Grb2. Since Grb2 is crucial to BCR-ABL signalling, the safety and efficacy of BP1001 in combination with tyrosine kinase inhibitors will also be studied in patients with advanced chronic myeloid leukaemia, including chronic myeloid leukaemia in blast phase. Furthermore, the favourable safety profile and encouraging pharmacodynamics of BP1001 suggest that the liposome-incorporated P-ethoxy antisense oligodeoxynucleotide approach could serve as a template to potentially target other so-called non-druggable proteins, including anti-apoptotic proteins and transcription factors. Contributors MO, GG-M, ML, SOB, YA, SV, WW, and JC enrolled patients. MO, ATA, SP, and JC collected data. MO, ATA, SP, and JC analysed the data. MO, ATA, and JC wrote the manuscript. GG-M, NP, TK, EJ, FR, GB, MA, MK, ML, SOB, YA, SV, WW, and HK reviewed and approved the manuscript. Declaration of interests ATA reports personal fees and other from Bio-Path Holdings Inc during the conduct of the study. ATA also has patent 7,309,692 (liposomal Grb2 antisense) licensed to Bio-Path Holdings Inc. JC reports grants and personal fees from Bio-Path Holdings Inc during the conduct of the study. All other authors declare no competing interests. Acknowledgments GG-M, MA, MK, WW, and HK are in receipt of an National Institutes of Health (NIH) grant, but this study was not funded by NIH and the authors are not employed by NIH.
Publisher Copyright:
© 2018 Elsevier Ltd
PY - 2018/4
Y1 - 2018/4
N2 - Background: Activating mutations of tyrosine kinases are common in leukaemias. Oncogenic tyrosine kinases use the growth factor receptor-bound protein 2 (Grb2) for signal transduction, leading to activation of mitogen-activated protein kinase (MAPK) 1 and MAPK3 (ERK2 and ERK1). We hypothesised that inhibition of Grb2 would suppress ERK1 and ERK2 activation and inhibit leukaemia progression. To inhibit Grb2, a liposome-incorporated antisense oligodeoxynucleotide that blocks Grb2 protein expression, BP1001, was developed. We report the first phase 1 findings of BP1001. Methods: In this single-centre, open-label, dose-escalation phase 1/1b trial, we enrolled participants (aged ≥18 years) with refractory or relapsed acute myeloid leukaemia, Philadelphia-chromosome-positive chronic myeloid leukaemia (in chronic, accelerated, or blast phase), acute lymphoblastic leukaemia, or myelodysplastic syndrome, at MD Anderson Cancer Center (Houston, TX, USA). We used a 3 + 3 dose escalation strategy, with at least three patients enrolled at each dose level. We administered BP1001 intravenously, twice weekly, for 28 days, with a starting dose of 5 mg/m2. If two or more patients developed toxic effects of grade 3 or higher, that dose level was deemed toxic. The dose was escalated if it did not produce dose-limiting toxic effects, and patients would be sequentially enrolled into cohort 2 (10 mg/m2), cohort 3 (20 mg/m2), cohort 4 (40 mg/m2), cohort 5 (60 mg/m2), or cohort 6 (90 mg/m2). After completion of monotherapy, we assessed the safety and toxicity of BP1001 (60 or 90 mg/m2) in combination with 20 mg low-dose cytarabine (twice-daily subcutaneous injections) in a phase 1b study in patients with refractory or relapsed acute myeloid leukaemia (ie, those who were refractory to at least one previous therapy regimen and no more than one previous salvage regimen). The objectives of this study were to establish the toxicity and tolerance of escalating doses of BP1001 monotherapy in patients with refractory or relapsed leukaemia, to assess the maximum tolerated dose of BP1001, and to determine the optimal biologically active dose of BP1001, defined as a 50% reduction in Grb2 expression in circulating leukaemia cells. We also aimed to assess the in-vivo pharmacokinetics of BP1001 and tumour response. The study is completed and is registered with ClinicalTrials.gov, number NCT01159028. Findings: Between July 23, 2010, and Feb 23, 2016, we enrolled and treated 39 patients, of whom 27 were assessable for dose-limiting toxicity. The first patient treated had mucositis and hand–foot syndrome, which were assessed as possibly related to BP1001 and counted as a dose-limiting toxicity. We noted no other dose-limiting toxicities, and a maximum tolerated dose was not identified. The highest tested dose of BP1001 was 90 mg/m2. The most common grade 3–4 adverse events were cardiopulmonary disorders (25 [64%] of 39 patients), and fever (including neutropenic fever) and infections (17 [44%] patients). Grade 5 adverse events were cardiopulmonary disorders (two [5%] of 39 patients), fever (including neutropenic fever) and infections (two [5%] of 39 patients), and multi-organ failure (one [3%] of 39 patients). Nine (33%) of 27 patients who had peripheral blood blasts at the start of therapy had a reduction of 50% or more in peripheral blood blasts while receiving BP1001 montherapy. Three (10%) of 29 patients who had bone marrow blasts at the start of therapy had a reduction in bone marrow blasts of 50% or more while receiving BP1001 monotherapy. Per investigator's assessment, seven (22%) of 32 patients benefited from BP1001 monotherapy and had extended cycles of treatment. Of seven patients receiving BP1001 plus low-dose cytarabine combination therapy, two had complete remission, one had complete remission with incomplete haematological recovery, and two had stable disease with no dose-limiting toxicity; one patient died and one withdrew, both because of disease progression. There were eight deaths; none were treatment related. Interpretation: BP1001 is well tolerated, with early evidence of anti-leukaemic activity in combination with low-dose cytarabine. To further explore this anti-leukaemic activity, the efficacy of BP1001 plus low-dose cytarabine combination is being investigated in an ongoing phase 2 study in patients with previously untreated acute myeloid leukaemia who are ineligible for intensive induction therapy. Funding: Bio-Path Holdings Inc.
AB - Background: Activating mutations of tyrosine kinases are common in leukaemias. Oncogenic tyrosine kinases use the growth factor receptor-bound protein 2 (Grb2) for signal transduction, leading to activation of mitogen-activated protein kinase (MAPK) 1 and MAPK3 (ERK2 and ERK1). We hypothesised that inhibition of Grb2 would suppress ERK1 and ERK2 activation and inhibit leukaemia progression. To inhibit Grb2, a liposome-incorporated antisense oligodeoxynucleotide that blocks Grb2 protein expression, BP1001, was developed. We report the first phase 1 findings of BP1001. Methods: In this single-centre, open-label, dose-escalation phase 1/1b trial, we enrolled participants (aged ≥18 years) with refractory or relapsed acute myeloid leukaemia, Philadelphia-chromosome-positive chronic myeloid leukaemia (in chronic, accelerated, or blast phase), acute lymphoblastic leukaemia, or myelodysplastic syndrome, at MD Anderson Cancer Center (Houston, TX, USA). We used a 3 + 3 dose escalation strategy, with at least three patients enrolled at each dose level. We administered BP1001 intravenously, twice weekly, for 28 days, with a starting dose of 5 mg/m2. If two or more patients developed toxic effects of grade 3 or higher, that dose level was deemed toxic. The dose was escalated if it did not produce dose-limiting toxic effects, and patients would be sequentially enrolled into cohort 2 (10 mg/m2), cohort 3 (20 mg/m2), cohort 4 (40 mg/m2), cohort 5 (60 mg/m2), or cohort 6 (90 mg/m2). After completion of monotherapy, we assessed the safety and toxicity of BP1001 (60 or 90 mg/m2) in combination with 20 mg low-dose cytarabine (twice-daily subcutaneous injections) in a phase 1b study in patients with refractory or relapsed acute myeloid leukaemia (ie, those who were refractory to at least one previous therapy regimen and no more than one previous salvage regimen). The objectives of this study were to establish the toxicity and tolerance of escalating doses of BP1001 monotherapy in patients with refractory or relapsed leukaemia, to assess the maximum tolerated dose of BP1001, and to determine the optimal biologically active dose of BP1001, defined as a 50% reduction in Grb2 expression in circulating leukaemia cells. We also aimed to assess the in-vivo pharmacokinetics of BP1001 and tumour response. The study is completed and is registered with ClinicalTrials.gov, number NCT01159028. Findings: Between July 23, 2010, and Feb 23, 2016, we enrolled and treated 39 patients, of whom 27 were assessable for dose-limiting toxicity. The first patient treated had mucositis and hand–foot syndrome, which were assessed as possibly related to BP1001 and counted as a dose-limiting toxicity. We noted no other dose-limiting toxicities, and a maximum tolerated dose was not identified. The highest tested dose of BP1001 was 90 mg/m2. The most common grade 3–4 adverse events were cardiopulmonary disorders (25 [64%] of 39 patients), and fever (including neutropenic fever) and infections (17 [44%] patients). Grade 5 adverse events were cardiopulmonary disorders (two [5%] of 39 patients), fever (including neutropenic fever) and infections (two [5%] of 39 patients), and multi-organ failure (one [3%] of 39 patients). Nine (33%) of 27 patients who had peripheral blood blasts at the start of therapy had a reduction of 50% or more in peripheral blood blasts while receiving BP1001 montherapy. Three (10%) of 29 patients who had bone marrow blasts at the start of therapy had a reduction in bone marrow blasts of 50% or more while receiving BP1001 monotherapy. Per investigator's assessment, seven (22%) of 32 patients benefited from BP1001 monotherapy and had extended cycles of treatment. Of seven patients receiving BP1001 plus low-dose cytarabine combination therapy, two had complete remission, one had complete remission with incomplete haematological recovery, and two had stable disease with no dose-limiting toxicity; one patient died and one withdrew, both because of disease progression. There were eight deaths; none were treatment related. Interpretation: BP1001 is well tolerated, with early evidence of anti-leukaemic activity in combination with low-dose cytarabine. To further explore this anti-leukaemic activity, the efficacy of BP1001 plus low-dose cytarabine combination is being investigated in an ongoing phase 2 study in patients with previously untreated acute myeloid leukaemia who are ineligible for intensive induction therapy. Funding: Bio-Path Holdings Inc.
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UR - http://www.scopus.com/inward/citedby.url?scp=85043538352&partnerID=8YFLogxK
U2 - 10.1016/S2352-3026(18)30021-8
DO - 10.1016/S2352-3026(18)30021-8
M3 - Article
C2 - 29550383
AN - SCOPUS:85043538352
SN - 2352-3026
VL - 5
SP - e136-e146
JO - The Lancet Haematology
JF - The Lancet Haematology
IS - 4
ER -
