Treatment of Philadelphia chromosome-positive acute lymphocytic leukemia with hyper-CVAD and imatinib mesylate

doi:10.1182/blood-2003-08-2958

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Blood, 15 June 2004, Vol. 103, No. 12, pp. 4396-4407.
Prepublished online as a Blood First Edition Paper on October 9, 2003; DOI 10.1182/blood-2003-08-2958.

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CLINICAL OBSERVATIONS, INTERVENTIONS, AND THERAPEUTIC TRIALS
Treatment of Philadelphia chromosome–positive acute lymphocytic leukemia with hyper-CVAD and imatinib mesylate
Deborah A. Thomas, Stefan Faderl, Jorge Cortes, Susan O'Brien, Francis J. Giles, Steven M. Kornblau, Guillermo Garcia-Manero, Michael J. Keating, Michael Andreeff, Sima Jeha, Miloslav Beran, Srdan Verstovsek, Sherry Pierce, Laurie Letvak, August Salvado, Richard Champlin, Moshe Talpaz, and Hagop Kantarjian
From the Departments of Leukemia, Pediatrics, Blood & Bone Marrow Transplantation, and Bioimmunotherapy, The University of Texas M. D. Anderson Cancer Center, Houston, TX; and Novartis Pharmaceuticals, East Hanover, NJ.

   Abstract

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Imatinib mesylate, an inhibitor of the Bcr-Abl tyrosine kinase,has modest activity in refractory/relapsed Philadelphia chromosome(Ph)-positive acute lymphocytic leukemia (ALL). Use of concurrentchemotherapy and imatinib mesylate in newly diagnosed Ph-positiveALL was explored. There were 20 patients who received hyper-CVAD(cyclophosphamide, vincristine, Adriamycin, and dexamethasone)and imatinib mesylate followed by imatinib mesylate-based consolidation/maintenancetherapy. Of these patients, 11 had de novo disease, 4 were primaryfailures after induction (without imatinib mesylate), and 5were in complete remission (CR) after induction (without imatinibmesylate). All 15 patients treated for active disease achievedCR. Within a median of 3.5 months in first CR, 10 patients underwentallogeneic stem cell transplantation (SCT). One patient relapsedafter matched related SCT. The other 9 patients remained alivein CR with median follow-up of 12 months after SCT (range, 1+to 17+ months). Among 10 patients ineligible for (no donor orolder age) or refusing allogeneic SCT, 1 patient relapsed afterone year. There were 5 patients who remained alive in continuousCR for a median of 20 months (range, 4+ to 24+ months), with2 older patients dying in CR at 15 and 16 months of comorbidconditions. Molecular CRs were achieved in both groups (SCTor no SCT). Outcome with hyper-CVAD and imatinib mesylate appearsbetter than with prior regimens; continued accrual and longerfollow-up of the current cohort is needed. (Blood. 2004;103:4396-4407)

   Introduction

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Philadelphia chromosome (Ph)-positive acute lymphocytic leukemia(ALL) is characterized by a reciprocal translocation betweenthe long arms of chromosomes 9 and 22 [t(9;22)(q34;q11)], leadingto the formation of the Bcr-Abl fusion protein. This translocationoccurs in about 3% to 5% of children and 20% to 30% of adultswith ALL, and is associated with a very poor prognosis.^1,2 Modernchemotherapy regimens for adult Ph-negative ALL result in completeresponse (CR) rates of 90% to 95% and long-term overall survival(OS) rates of 35% to 40%.^3-7 Despite achievement of similarlyhigh CR rates of 80% to 90% with these chemotherapy regimens,most patients with Ph-positive ALL relapse and die from thedisease.^8-10 The 5-year survival rates are less than 10% foradults. Children with Ph-positive ALL treated with chemotherapyalone have higher survival rates of 25% to 30%, but worse outcomesare seen with leukocyte counts higher than 100 x 10⁹/L and/orfailure to respond to glucocorticoid therapy.^11,12 Allogeneicstem cell transplantation (SCT) in first CR can increase thelong-term event-free survival (EFS) rate to 28% to 40% for adultsand to 60% to 75% for children.^11,13-18
The unique biologic behavior of Ph-positive ALL is attributedto molecular changes resulting from the Abl proto-oncogene fromchromosome 9 fusing within the 5' half of the breakpoint clusterregion (bcr) sequences on chromosome 22.^19,20 The chimeric Bcr-Abloncogene leads to fusion proteins of different sizes dependingon the location of the Bcr breakpoint. If the break within thefirst intron of BCR (m-bcr region) splices the first exon ofthe BCR gene to the second exon of the ABL gene (e1a2), the190 kDa fusion oncoprotein is generated. This oncoprotein (p190^bcr-abl)occurs in 60% to 80% of patients with Ph-positive ALL; the other20% to 40% are characterized by the larger p210^bcr-abl fusiononcoprotein typical of chronic myelogenous leukemia (CML). Thelatter is formed when exon b2 or exon b3 of the BCR gene (M-bcrregion) is coupled to ABL exon 2 (b2a2 or b3a2 junction). Gleissneret al²¹ reported an association of the p210^bcr-abl subtype witholder age and trend toward worse 3-year survival rates, althoughmost studies have not demonstrated differences in clinical presentationor outcome with either p190^bcr-abl or p210^bcr-abl ALL.^21-24
These Bcr-Abl molecular abnormalities may be sufficient forleukemic transformation as demonstrated in animal models showinga p210^bcr-abl tyrosine kinase-dependent development of a CML-likedisease.²⁵ The mechanism of leukemogenesis appears related tothe constitutively activated and dysregulated tyrosine kinaseactivity that results in downstream effects on multiple signaltransduction pathways controlling cellular proliferation andapoptosis.²⁶ Imatinib mesylate (Gleevec, STI571; Novartis PharmaceuticalsCorporation) is a selective inhibitor of the Bcr-Abl tyrosinekinase, platelet-derived growth factor (PDGF) receptor tyrosinekinase, and the c-kit receptor kinase.²⁷ In vitro, imatinibmesylate inhibited the growth of Bcr-Abl-positive cells by inducingapoptosis and suppressing proliferation.^28-30 In clinical trials,imatinib mesylate demonstrated significant anti-CML activityand is now a standard frontline treatment in newly diagnosedPh-positive CML.^31-39 Single-agent imatinib mesylate therapyfor previously treated relapsed or refractory Ph-positive ALLand CML in lymphoid blast phase was associated with objectiveresponse rates of 40% to 50%; true CR rates (lasting for 4 weeksor more) were 5% to 7% with the median survival of 2 to 5 months.^39-41
Mechanisms of resistance such as Bcr-Abl amplification or mutationsin the Bcr-Abl tyrosine kinase have been identified in previouslytreated Ph-positive ALL patients salvaged with single-agentimatinib mesylate.^42,43 These results suggest that use of imatinibmesylate as a single agent in Ph-positive ALL is unlikely tobe sufficient for long-term disease control. In vitro studiessuggest synergistic activity of imatinib mesylate with chemotherapyagents such as anthracyclines, vincristine, and cytarabine (ara-C).^44,45This report summarizes the experience with hyper-CVAD (cyclophosphamide,vincristine, Adriamycin, and dexamethasone),⁴⁶ a dose-intensivechemotherapy regimen used at our institution for adult ALL since1992, and imatinib mesylate for patients with de novo Ph-positiveALL.

   Patients and methods

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Eligibility
Adults (age 15 years or older) with Ph-positive ALL, newly diagnosedor minimally treated, were entered on the institutional reviewboard-approved study after informed consent was obtained accordingto institutional guidelines. Patients previously treated withinduction chemotherapy without imatinib mesylate (either failingafter 1 course or in CR after up to 2 courses of therapy withoutimatinib mesylate) were eligible. Entry criteria included EasternCooperative Oncology Group (ECOG) performance status 0 to 2,adequate renal and hepatic functions (serum creatinine <176.8 µM [2 mg/dL] and bilirubin < 34.2 µM [2mg/dL]), and adequate cardiac status (New York Heart Associationclass III-IV excluded). Patients with uncontrolled serious infectionsor active secondary malignancy that was thought to shorten survivalto less than one year were not eligible. No investigationalantileukemic therapy could have been administered within theprior 7 days. Patients must have been willing to practice contraception.
Therapy
Therapy was given with 8 induction-consolidation courses alternatinghyper-CVAD with high-dose methotrexate (MTX) and cytarabine(ara-C), concurrently with imatinib mesylate.
Briefly, the treatment regimen was as follows. Imatinib mesylatewas given at the standard dose of 400 mg orally daily on days1 to 14 of each of the intensive chemotherapy courses, withoutresumption until the next course to allow recovery from myelosuppression.Odd courses (nos. 1, 3, 5, and 7) were hyper-CVAD: hyper-fractionatedcyclophosphamide (CTX) given 300 mg/m² intravenously over 2hours every 12 hours for 6 doses on days 1 to 3 with 600 mg/m²Mesna per day intravenously via continuous infusion on days1 to 3 beginning 1 hour prior to CTX and completed by 12 hoursafter the last dose of CTX; 2 mg vincristine intravenously ondays 4 and 11; 50 mg/m² doxorubicin (Adriamycin) intravenouslyover 24 hours via central venous catheter on day 4 (given over48 hours in patients with reduced ejection fractions < 50%);and 40 mg dexamethasone daily either orally or intravenouslyon days 1 to 4 and days 11 to 14. Granulocyte colony-stimulatingfactor (G-CSF, 10 µg/kg [rounded]) was initiated approximately24 hours after completion of chemotherapy until the absoluteneutrophil count (ANC) was higher than 1 x 10⁹/L.
The first course was accompanied by appropriate intravenoushydration and alkalinization (eg, dextrose water or one-halfnormal saline with 75 to 100 milliequivalents of sodium acetateper liter to run at 50 to 100 mL/h) and allopurinol to reducethe incidence of tumor lysis syndrome. Oral sodium bicarbonatesupplemented the intravenous formulation on days 1 to 3. Rasburicasecould be substituted for allopurinol in cases with high whiteblood cell count at presentation.
Even courses (nos. 2, 4, 6, and 8) included high-dose MTX andara-C: 1 g/m² MTX intravenously over 24 hours on day 1; and3 g/m² (1 g/m² in patients aged 60 or older) ara-C over 2 hoursevery 12 hours for 4 doses on days 2 and 3 were given. Intravenousalkalinization was used to promote excretion of MTX in all courses(as for course 1 at a rate of 100 to 125 mL/h). Calcium leucovorinwas given at a dose of 50 mg intravenously starting 12 hoursafter the completion of MTX and continued at a dose of 15 mgintravenously every 6 hours for 8 doses until MTX blood levelswere less than 0.1 µM. An algorithm of additional leucovorinrescue (50 mg intravenously every 6 hours) was followed if MTXblood levels were elevated at 0 hour (at end of infusion andconfirmed on repeat sample), more than 20 µM; 24 hours,more than 1 µM; and 48 hours, more than 0.1 µM.Oral acetazolamide was used if the urine pH was less than 7.0to promote excretion. G-CSF was repeated as for the odd courses.
Central nervous system (CNS) prophylaxis included alternatingintrathecal therapy with 12 mg MTX (6 mg only if via ommaya)on day 2 and 100 mg ara-C on day 7 or 8 of each course for eithera total of 6 or 8 intrathecal treatments, depending on riskfor CNS relapse (based on serum lactate dehydrogenase [LDH]level > 1400 U/L and/or proliferative index %S + G₂M $≥$ 14%).⁴⁷Therapy for active CNS leukemia at presentation included anincrease in frequency of the alternating intrathecal therapyduring the induction course to twice weekly until the CSF cellcount normalized and the cytologic examination was negativefor evidence of malignant cells. Intrathecal therapy was thenadministered weekly for 4 weeks; then the prophylactic schedule(2 intrathecals per course) was resumed for the remaining coursesof intensive chemotherapy. No prophylactic cranial irradiation(XRT) was administered. Therapeutic XRT was given if indicatedfor CNS disease at presentation (eg, cranial nerve palsies withXRT to the base of the skull).
All de novo (n = 11) or primary refractory (n = 4) patientsbegan imatinib mesylate treatment with course 1, whereas 5 previouslytreated patients started protocol therapy with course 2, sincethey had received hyper-CVAD or anthracycline-based chemotherapy(without imatinib mesylate) as induction therapy. Eligible patientsin first CR were referred for allogeneic SCT as soon as feasibleafter treatment was initiated.
Following completion of the 8 courses of intensive chemotherapy,maintenance therapy was planned for 13 months and consistedof 600 mg imatinib mesylate orally daily, 2 mg vincristine intravenouslyevery month, and 200 mg prednisone daily for 5 days every month(commenced the day of the vincristine infusion). Higher dosesof imatinib mesylate were given owing to the known dose-responsephenomenon observed in the studies of imatinib mesylate in CMLand the absence of concurrent myelosuppressive therapy.³¹ Maintenancetherapy was interrupted during months 6 and 13 with hyper-CVADand imatinib mesylate intensifications given as with prior coursesof intensive chemotherapy.
Dose reductions included the following: (1) ara-C decreasedto 1 g/m² for age 60 years or older, creatinine level higherthan 2 g/dL, or MTX level at 0 hour (repeated) higher than 20µM; (2) vincristine to 1 mg for total bilirubin higherthan 2 g/dL; (3) vincristine eliminated if above total bilirubinhigher than 3 g/dL or grades 3 to 4 peripheral neuropathy orileus; (4) doxorubicin decreased by 50% for bilirubin 2 to 3g/dL, by 75% for bilirubin 3 to 5 g/dL, and eliminated for bilirubinhigher than 5 g/dL; (5) MTX decreased by 50% for calculatedcreatinine clearance 10 to 50 mL/min, with decrease by 25% to50% for delayed excretion, nephrotoxicity, or grade 3 or greatermucositis with prior courses. Imatinib mesylate was reducedto 300 mg for grades 3 to 4 hepatotoxicity during intensivechemotherapy courses (400 mg if during maintenance).
Supportive care
Oral prophylactic antibiotic therapy included either a quinolone(500 mg ciprofloxacin twice daily or 500 mg levofloxacin daily)or trimethoprim-sulfamethoxazole one double strength twice dailyfor antibacterial coverage, 200 mg fluconazole daily for antifungalcoverage, and 200 mg acyclovir twice daily (or 500 mg valacyclovirdaily) for mucositis prophylaxis with antiviral coverage. Hematologicprofiles were obtained at least weekly. Appropriate transfusionsupport was provided with packed red blood cells given for symptomaticand/or severe anemia. Platelet transfusions were given prophylacticallyfor platelet counts lower than 10 to 15 x 10⁹/L or therapeuticallyfor platelet count lower than 30 to 50 x 10⁹/L with hemorrhage.All blood products were irradiated. Neutropenic febrile episodesgenerally resulted in hospitalization and initiation of broadspectrum parenteral antibiotics.
Assessments
Pretreatment evaluations included history and physical examination,complete blood count with differential, Sequential MultipleAnalysis-12, and bone marrow aspiration for histology, flowcytometry, and cytogenetic studies. Cytogenetic analysis wasperformed by standard techniques, with bone marrow specimensexamined on direct or short-term (24-hour) cultures.⁴⁸ Fluorescentin-situ hybridization (FISH) and quantitative real-time polymerasechain reaction (RT-PCR) assays for bcr-abl were performed onmarrow samples of patients who were in complete remission whenfeasible by methods detailed previously.⁴⁹ RT-PCR was confirmedby nested PCR when negative.
Marrow aspirations were repeated approximately day 14 and day21 of course 1 in patients with active disease at study entry,with the latter sample assessed for cytogenetics, FISH, andquantitative RT-PCR. Complete blood counts were performed atleast weekly during the intensive courses of chemotherapy. Analysesof renal and hepatic function were performed prior to each cycleof chemotherapy. Bone marrow aspirations were repeated every2 to 3 courses.
Baseline cardiac function was assessed by echocardiogram ormulti-gated radionuclide ventriculography (MUGA) in patientswith cardiac risk factors, and repeated in cases where clinicalsymptoms were reported or in preparation for allogeneic SCT.The presence or absence of CNS disease was evaluated in allpatients concurrently with administration of CNS prophylaxiswith methotrexate (approximately day 2 of the first course).Cerebrospinal fluid was assessed by cell count with differentialand cytologic evaluation.
Response criteria
Complete remission (CR) was defined as 5% or less blasts ina normocellular or hypercellular marrow with a granulocyte countof 1.0 x 10⁹/L or higher and platelet count of 100 x 10⁹/L orhigher. Complete resolution of extramedullary disease was requiredfor CR. Molecular CR was defined as achievement of RT-PCR negativityin addition to hematologic criteria for CR. Other response outcomeswere defined as induction death (if occurring after start oftherapy without meeting the definition of CR or resistant disease)and resistant disease (if the patient survived the inductiontreatment period but the leukemia persisted or regrew). Relapsewas defined as disease recurrence at any site after achievingCR.
Statistical considerations
The characteristics and treatment results of the de novo patientswere compared with the historical control group of patientswith Ph-positive ALL treated with either VAD (vincristine, doxorubicin,and dexamethasone) regimens⁵⁰ from 1983 until 1991, or withhyper-CVAD with or without rituximab from 1992 until 2000.^46,51Differences in response rates by pretreatment characteristicsamong subgroups were analyzed by ${chi}$ ² or Fisher exact tests.⁵²Survival was measured from the date of initiation of therapyuntil death from any cause. Disease-free survival was measuredfrom the date of CR until documented relapse. Survival and disease-freesurvival curves were plotted according to the methods of Kaplanand Meier, with differences among them analyzed by the log-ranktest.⁵³ Toxicity was evaluated according to the National CancerInstitute Expanded Common Toxicity Criteria (version 2.0).

   Results

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Study group
From April 2001 to March 2003, 20 patients with newly diagnosedPh-positive ALL were entered in the study. Of the patients,11 (55%) presented with de novo disease, 4 (20%) were refractoryto standard induction chemotherapy, and 5 (25%) entered thestudy in CR after one course of induction chemotherapy (allbut 1 with minimal residual disease detectable by FISH and/orPCR). The p190^bcr-abl was expressed in 50% of the patients,with p210^bcr-abl in the remainder. The median age of the groupwas 42 years (range, 17 to 75 years); 70% were males. Characteristicsof this group were compared with 31 de novo Ph-positive ALLpatients treated with VAD⁵⁰ and with 50 patients treated withthe hyper-CVAD regimen with or without rituximab^46,51 (Table 1).Patients in the hyper-CVAD and imatinib mesylate group hada lower incidence of elevated ${beta}$ ₂ microglobulin and LDH levels;however, they had a higher incidence of adverse features suchas CNS disease and lower albumin levels compared with patientstreated with prior regimens.

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Table 1.. Characteristics and response of Philadelphia-positive ALL study groups

Response
All 15 patients (100%) treated with active disease achievedCR. The CR rates after one cycle of induction therapy were 52%for VAD, 66% for hyper-CVAD with or without rituximab, and 93%for hyper-CVAD and imatinib mesylate (P < .01). Overall CRrates reflected the number of patients who required more thanone course to achieve morphologic and hematologic CR (16%, 30%,and 7%, respectively). The median times to CR for the 3 regimens(24, 20, and 19 days); ANC recovery of 1 x 10⁹/L or higher (22,23, and 20 days); and platelet count of 100 x 10⁹/L or higher(24, 25, and 21 days) were shorter overall for the hyper-CVADand imatinib mesylate regimen, although this did not reach statisticalsignificance (Table 1).
Bone marrow cytogenetics performed at CR (approximately day21 of the induction course) showed normalization to diploidkaryotype in 13 (87%) of the 15 patients. Levels of marrow quantitativeRT-PCR positivity (ratio of bcr-abl/abl x 100) less than 0.05occurred in 8 patients with the hyper-CVAD and imatinib mesylateregimen alone (Table 2). Complete molecular remission (confirmedby nested PCR) was achieved in 5 patients after hyper-CVAD andimatinib mesylate alone (patient nos. 2, 12, 13, 14, 17), andin 12 (60%) of 20 patients overall. For patients unwilling orunable to undergo allogeneic SCT, serial assessments of quantitativeRT-PCR demonstrated stable to decreasing levels of Bcr-Abl transcriptsover time, particularly with initiation of higher dose imatinibmesylate during maintenance therapy (Table 2).

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Table 2.. Minimal residual disease marrow assessments with hyper-CVAD and imatinib mesylate

Remission duration and survival
The median follow-up of the study group is 20 months (range,4+ to 24+ months). All but 5 of the 20 patients remained alivein CR with hyper-CVAD and imatinib mesylate-based therapy (9/10after hyper-CVAD and imatinib mesylate followed by allogeneicSCT, 6/10 after hyper-CVAD and imatinib mesylate alone) (Figure 1).Of the deaths with hyper-CVAD and imatinib mesylate withor without SCT, 2 were related to ALL relapse. The first deathwas a 28-year-old female (patient no. 1) with primary refractorydisease (failure to induction chemotherapy with the "Linkerregimen" and active CNS disease at presentation) who had simultaneousmarrow and CNS relapse 12 months from study entry despite continuanceon maintenance therapy (refused allogeneic SCT). The patientsubsequently failed multiple salvage regimens and died of Aspergilluspneumonia prior to planned matched unrelated donor (MUD) SCT.The second death was a 57-year-old male (patient no. 7) withde novo disease who underwent matched related allogeneic SCTafter 3 courses of hyper-CVAD and imatinib mesylate, and relapsedon day 160 of SCT (9 months from start of hyper-CVAD and imatinibmesylate) with marrow and CNS disease (had completed CNS prophylaxisfor low-risk disease). The patient succumbed to complicationsof probable fungal pneumonia on day 26 of reinduction therapywith hyper-CVAD and imatinib mesylate.

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Figure 1.. Disease-free survival of patients treated with hyper-CVAD and imatinib mesylate compared with those treated with non-imatinib mesylate-containing hyper-CVAD and VAD regimens. Note: a long-term survivor at 15 years in the VAD group is not shown.

Of the deaths, 2 occurred in patients who had maintained continuousCR. The first was a 75-year-old male (patient no. 13) who diedin CR after 15 months related to sequelae of osteomyelitis fromvertebroplasty for trauma-related vertebral fracture (with underlyingosteoporosis). The second death was in a 55-year-old female(patient no. 14) with underlying diabetes mellitus who diedin CR after 16 months related to sequelae of sinus infectionwith mucormycosis unresponsive to antifungal therapy.
There were 2 patients who discontinued protocol therapy forpersistence or recurrence of Ph-positive disease by routinekaryo-typing without evidence of overt ALL. One 46-year-oldfemale (patient no. 6) subsequently relapsed 5 months later(11 months from diagnosis) despite treatment with higher doseimatinib mesylate concurrently with an asparaginase-containingregimen. Salvage therapy regimen was given without success,with demise resulting from complications of matched unrelateddonor allogeneic SCT and recurrent disease (Figure 2). The otherpatient (no. 16) remained on single-agent high-dose imatinibmesylate for 5+ months (12 months from diagnosis) with persistenceof Ph-positive metaphases in the marrow without recurrence ofALL at the time of this report.

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Figure 2.. Overall survival of patients treated with hyper-CVAD and imatinib mesylate compared with those treated with non-imatinib mesylate-containing hyper-CVAD and VAD regimens. Curves represent intention to treat, without censoring for allogeneic SCT. Differences remain significant with exclusion of the 5 patients in CR at start of hyper-CVAD and imatinib mesylate (not shown). Note: a long-term survivor at 15 years in the VAD group is not shown.

There were 2 patients who had completed all therapy per currentprotocol, including both intensifications during maintenancetherapy, without proceeding to allogeneic SCT. Both remainedin continuous CR but were placed on alternate therapy afterstudy completion. The first was a 66-year-old male (patientno. 2) who achieved RT-PCR negativity and was initially observed,declining nonmyeloablative allogeneic SCT. Surveillance marrowassessment performed 3 months after discontinuing therapy showedcontinued CR with detectable RT-PCR transcripts. He resumedmaintenance therapy with imatinib mesylate, vincristine, andprednisone. The second is a 53-year-old female (patient no.5) without an identifiable stem cell transplant donor who remainedRT-PCR positive and was continued on maintenance therapy withhigh-dose imatinib mesylate and prednisone (without vincristinebecause of peripheral neuropathy).
Figures 1 and 2 illustrate the respective DFS and survival ofpatients treated with hyper-CVAD and imatinib mesylate comparedwith those treated with non-imatinib mesylate-containing hyper-CVADor VAD regimens. DFS and survival of the study group with currentfollow-up was not different whether patients were censored oruncensored at the time of allogeneic SCT (data not shown). Figures3 and 4 show the DFS and survival by disease status prior tostart of therapy (eg, de novo, CR at start, or primary refractory).

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Figure 3.. Disease-free survival of Ph-positive ALL by status of disease at study entry for those treated with hyper-CVAD and imatinib mesylate. One de novo relapsed after allogeneic SCT (patient no. 7), one CR at start relapsed after change in therapy (patient no. 6), and one primary refractory (patient no. 1) relapsed on therapy without SCT. Deaths in complete remission (one de novo, one primary refractory) are censored.

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Figure 4.. Survival by disease status at study entry. Deaths were related to relapse in patient nos. 7, 6, and 1 (one de novo after allogeneic SCT, one CR at start after change in therapy, one primary refractory while on therapy) or other causes while in CR for one de novo and one primary refractory (patient nos. 14, 13).

Allogeneic stem cell transplantation
There were 10 patients (50%) who underwent allogeneic SCT infirst CR at a median time of 3.5 months (range, 1-8 months)from start of therapy. Of the 10 patients who did not undergoSCT, reasons were lack of donor or older age (n = 5), persistence/recurrenceof Ph-chromosome without leukemia (n = 2), and/or refusal ofprocedure (n = 3). Allogeneic SCT in first CR was performedat M. D. Anderson Cancer Center in all cases. Conditioning regimensincluded CTX, rituximab, and total body irradiation (TBI) (n= 4); CTX and TBI (n = 3); CTX, alemtuzumab, and TBI (n = 2);or fludarabine and TBI (n = 1). Donor sources were matched relatedsibling (n = 8), matched unrelated donor (n = 1), and cord blood(n = 1). Of the 10 patients (90%) who underwent allogeneic SCT,9 remained alive in CR with a median time from allogeneic SCTof 12 months (range, 1-17 months). Imatinib mesylate (dailydoses ranging from 100 to 400 mg) was resumed after allogeneicSCT as maintenance therapy in 4 patients (usually commencedafter full hematologic recovery from SCT).
Mild to moderate graft-versus-host disease (GVHD) was observedin 5 patients. One de novo patient (no. 7) undergoing matchedrelated allogeneic SCT after 3 courses of chemotherapy withhyper-CVAD and imatinib mesylate relapsed on day 160 of SCTwith bone marrow and CNS disease (received CNS prophylaxis forlow-risk disease). Conversion to RT-PCR negativity (confirmedby nested PCR) was observed in 8 of 9 patients who were RT-PCRpositive prior to allogeneic SCT (patient no. 18 after allogeneicSCT quantitative RT-PCR pending, patient no. 17 negative forBcr-Abl by nested PCR prior to SCT).
Results of SCT in first CR with Ph-positive ALL patients treatedprior to hyper-CVAD and imatinib mesylate included 5 (16%) of31 patients previously treated with VAD chemotherapy from 1981to 1992. Median time to SCT was 3 months (range, 2 to 7 months).Conditioning regimen for all 5 patients was etoposide, CTX,and TBI. Of the patients, 2 were consolidated with autologousSCT and 3, with matched related sibling SCT; 2 patients diedfrom infectious complications of allogeneic SCT, and 2 patientsdied after relapse at 4 and 8 months after SCT. One patientremained alive without evidence of disease after the autologousintensification at 15 years (not shown in Figures 1, 2).
Of 50 patients treated with hyper-CVAD without imatinib mesylate,12 (24%) underwent SCT in first CR, within a median time of4 months (range, 1-7 months). No autologous SCTs were performedin this group. Conditioning regimens included CTX and TBI (n= 5); etoposide, CTX, and TBI (n = 3); thiotepa, CTX, and TBI(n = 3); or CTX, rituximab, and TBI (n = 1). Matched relatedsibling donors were used in 7, matched unrelated donors in 4,and 1-antigen mismatch related donor in 1 patient. Of the patients,4 died in CR related to infectious complications or GVHD; 6relapsed a median time of 6 months from SCT (range, 2 to 38months); and 2 remained alive without evidence of disease at45 and 60 months from SCT. Overall, 7 patients (58%) had mildacute or chronic GVHD.
Toxicity
The median time to hematologic recovery after each cycle ofchemotherapy with the hyper-CVAD and imatinib mesylate regimenwas not significantly different from the prior non-imatinibmesylate regimens. Median time to complete remission was 19days (range, 15-22 days; Table 1). The median time to recoveryvaried by cycle with each of the subsequent courses of consolidationtherapy. The median time to neutrophil recovery to ANC of 10⁹/Lor higher for the odd cycles (hyper-CVAD) ranged from 12 to28 days, and 12 to 24 days for the even cycles (high-dose methotrexateand ara-C). The median time to recovery of the platelet countto 50 x 10⁹/L or higher ranged from 14 to 21 days for the oddcycles, and 13 to 37 days for the even cycles. The incidenceof febrile episodes and documented infections was similar amongthe 3 programs. No induction mortality was observed. Toxicitiesobserved with the hyper-CVAD and imatinib mesylate combinationwere not significantly different from the prior regimens, withthe majority of expected events related to each of the chemotherapycomponents of the regimen. Toxicities observed with the hyper-CVADand imatinib mesylate regimen are summarized in Table 3.

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Table 3.. Toxicities of hyper-CVAD and imatinib mesylate in 91 postinduction courses

   Discussion

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Outcome with conventional chemotherapy programs for adults withPh-positive ALL has been poor (Table 4).^7,22,54-66 Remissionrates have ranged from 46% to 90%, with median remission durationsof 6 to 11 months. Overall 3-year survival rates without allogeneicSCT are less than 20%, and reach only 30% to 40% with SCT inselected patients. The hyper-CVAD regimen, although effectivein producing high CR rates similar to the non-Ph-positive counterparts,has not improved long-term DFS or overall survival in Ph-positiveALL.

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Table 4.. Outcome with conventional chemotherapy for adults with Ph-positive ALL

In our study, we treated 20 patients with de novo Ph-positiveALL with a combination of hyper-CVAD and imatinib mesylate.All 15 patients with active disease at the start of therapyachieved CR. With a median follow-up of 20 months, 15 patients(75%) were alive without evidence of ALL. Of the 20 patients,10 (50%) were able to undergo allogeneic SCT. With a medianfollow-up of 12 months after allogeneic SCT, all but 1 of these10 patients remained alive without disease. Outcome in the 10patients who had not undergone allogeneic SCT (for reasons oflack of donor, older age, prohibitive comorbid conditions, orrefusal) included 6 patients who remained alive without diseaseafter a median follow-up of 20 months (1 primary refractorypatient relapsed at 12 months, 1 patient relapsed after changefrom hyper-CVAD and imatinib mesylate to alternate therapy forpersistent Ph-positive metaphases at 10 months, and 2 patientsdied in CR at 15 and 16 months related to comorbid conditions).
Outcome with the hyper-CVAD and imatinib mesylate regimen issignificantly better than the historical control group treatedwith VAD⁵⁰ (n = 31) or hyper-CVAD without imatinib mesylate^46,51(n = 50) with respect to CR rates (P < .01), DFS (P <.001), and overall survival rates (P = .001) (Table 1; Figures1, 2). With current follow-up of the study group, neither medianremission duration nor median survival has been reached. Therewas no significant difference in survival or DFS with censoringat the time of allogeneic SCT. The regimen was tolerable, withtoxicity profile of the hyper-CVAD and imatinib mesylate combinationsimilar to that of hyper-CVAD alone (Tables 1, 3). The historicalrate of proceeding to allogeneic SCT in first CR for Ph-positiveALL at our institution was 20% with prior ALL programs, comparedwith 50% in this study. Several factors could account for theincreased success of performing allogeneic SCT in first CR,including increased availability of unrelated donors, timelinessof referral for consideration of transplantation, and longerduration of remission allowing time for potential search fordonors and eventual SCT.
Allogeneic SCT in Ph-positive ALL in first CR remains the standardintervention until optimal uses and long-term results of imatinibmesylate in combination with chemotherapy are known. Publishedseries of allogeneic SCT in adults have shown DFS rates rangingfrom 31% to 65% and survival rates of 37% to 72% (Table 5).^{11,14-16,18,66-70}In a large prospective randomized trial of 167 patients withPh-ALL treated between 1993 and 2000 on UKALL12/ECOG 2993 protocols,88 patients (53%) received chemotherapy alone, 49 (29%) underwentMRS SCT in first CR, 23 (14%) had an MUD SCT, and 7 (4%) receivedautologous intensification.¹⁸ The actuarial 5-year relapse riskwas lower with allogeneic SCT (related or unrelated donor) comparedwith chemotherapy or autologous SCT (32% versus 81%, P <.0001). Allogeneic SCT was also associated with a better 5-yearDFS rate (36% versus 17%, P = .02) and survival rate (42% versus19%, P = .02) compared with chemotherapy. Dombret et al⁶⁶ reportedsimilar results in a prospective study of LALA-94 chemotherapywith planned allogeneic SCT in 154 patients with Ph-positiveALL. All patients with a matched related or unrelated donorwere assigned to allogeneic SCT; those without a donor underwentautologous SCT. The availability of a donor and absence of minimalresidual disease (MRD) prior to SCT were both associated withlonger DFS (P < .001 and P = .01, respectively) and survival(P = .02 and P = .01, respectively). The 3-year survival rateswere 37% for the donor group versus 12% for the no-donor group(P = .02). The role of SCT after hyper-CVAD and imatinib mesylateremains to be determined, as durable remissions were observedwith hyper-CVAD and imatinib mesylate alone.

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Table 5.. Outcome with allogeneic stem cell transplantation in Philadelphia-positive acute lymphocytic leukemia

Sensitive quantitative RT-PCR techniques enable detection ofa single leukemia cell in 10⁴ to 10⁶ normal cells. In Ph-positiveALL, the level of residual leukemia has predicted the probabilityof relapse after allogeneic SCT.^10,23,71-74 Radich et al²⁴ reporteda significantly increased relapse risk in patients with a positivePCR for Bcr-Abl after transplantation (relapse rate 43%) comparedwith patients with negative PCR. Return to negative RT-PCR statushas been reported after the development of chronic GVHD, suggestinga graft-versus-leukemia (GVL) effect, with decreased incidenceof relapse compared with patients who did not develop chronicGVHD (15% versus 100%, P = .01).⁷¹ Serial measurements of quantitativePCR for Bcr-Abl in patients with relapsed or refractory Ph-positiveALL treated with single-agent imatinib mesylate showed medianreductions in Bcr-Abl/glyceraldehydes-3-phosphate dehydrogenase(GAPDH) ratios of 2 to 3 logs, with lower Bcr-Abl levels (<10^-2) correlating with longer time to progression.⁷⁵ In anotherstudy, a higher log-reduction of Bcr-Abl levels over time wasnoted in patients treated with single-agent imatinib mesylatecompared with those treated with chemotherapy, attributed tothe high specificity of this agent.⁷⁶
In our study, serial monitoring of MRD by quantitative RT-PCRdemonstrated detectable transcripts in some patients treatedwith hyper-CVAD and imatinib mesylate (Table 2). Overall, 12(60%) of 20 patients remained RT-PCR negative and 10 (66%) of15 patients remained negative for Bcr-Abl by FISH, without relapsesobserved to date after achieving RT-PCR-negative status exceptin one patient after SCT (who became FISH positive prior torelapse). The proportion of patients with the e1a2 (p190^bcr-abl)or b3a2 (p210^bcr-abl) was approximately equal, and no differenceswith respect to response or outcome were observed. Despite achievementof molecular remission by RT-PCR after hyper-CVAD and imatinibmesylate followed by unmaintained allogeneic SCT, relapse wasobserved. There were 3 other failures: 1 patient with p190^bcr-ablALL with overt relapse on maintenance therapy and 2 patientswith p210^bcr-abl ALL with persistence or recurrence of Ph-positivemetaphases during intensive chemotherapy.
Potential reasons for the hyper-CVAD and imatinib mesylate failuresin our study include development of resistance by mechanismsreported previously (eg, mutations in the adenosine triphosphate[ATP]-binding domain of Abl, amplification of the Bcr-Abl gene,and/or up-regulation of Bcr-Abl transcription).^42,43,77 Alternativescould be pharmacologic interactions that decreased drug levelsof imatinib mesylate (metabolized via cytochrome P450).^44,45The minimum level of imatinib mesylate required for 50% inhibitionof cellular phosphorylation of Bcr-Abl is 0.25 µM. Invivo animal studies have shown that imatinib mesylate penetratedthe blood-brain barrier poorly.⁷⁸
Analysis of CSF levels of imatinib mesylate in patients treatedwith single-agent imatinib mesylate for Ph-positive ALL or CMLin lymphoid blast crisis have shown average CSF imatinib mesylatelevels in the subtherapeutic range (0.88 µM).⁷⁹ Thus,concurrent intrathecal CNS prophylaxis should be administeredto all patients with de novo Ph-positive ALL, as was done inour study. No isolated CNS relapse had been observed at thetime of this report.
The success of our study, in part, has been to increase theproportion of patients able to undergo allogeneic SCT comparedwith historical rates. Although 10 patients were unable to undergoallogeneic SCT, it is possible that long-term remission statuscan be achieved in the absence of SCT (2 patients treated withhyper-CVAD and imatinib mesylate alone remain in complete cytogeneticremission for more than 2 years with continuation of imatinibmesylate-based maintenance therapy). Longer follow-up of theseand other cohorts unable to undergo allogeneic SCT will be requiredto determine the optimal therapeutic strategy in Ph-positiveALL.
Future directions include consideration of pharmacokinetic assaysduring therapy to determine the effects of various componentsof the chemotherapy on imatinib mesylate levels to ensure optimaldose delivery. Given the tolerance of the regimen to date, anddose-response relationship observed in Ph-positive CML, increasedduration of exposure and dosing of imatinib mesylate with chemotherapyis under investigation. The addition of rituximab to the hyper-CVADand imatinib mesylate regimen in patients with CD20 expressionwill be studied, given the preliminary favorable results observedwith the hyper-CVAD and rituximab regimens in de novo ALL andBurkitt leukemia/lymphoma.⁵¹ Use of imatinib mesylate with orwithout rituximab as maintenance therapy after allogeneic SCTshould be studied prospectively. The significance of MRD inrelation to relapse and prognosis will need to be determinedto guide therapeutic modifications. Enrollment of patients intoclinical trials will be crucial to furthering our knowledgeregarding the role of imatinib mesylate in the treatment ofde novo Ph-positive ALL.

   Acknowledgements

Imatinib mesylate was supplied by Novartis Pharmaceuticals Corporationto the participants of this study free of charge.

   Footnotes

Submitted September 2, 2003; accepted September 29, 2003.
Prepublished online as Blood First Edition Paper, October 9,2003; DOI 10.1182/blood-2003-08-2958.

Supported in part by the National Institutes of Health (NIH)grant 5K12 CA88084-2.

Presented in part at the 43rd and 44th Annual Meeting of theAmerican Society of Hematology, Orlando, FL and Philadelphia,PA, respectively, and the 39th Annual Meeting of the AmericanSociety of Clinical Oncology, Chicago, IL.^80-82

Two of the authors (L.L., A.S.) are employed by Novartis PharmaceuticalsCorporation, whose product was studied in the present work.

An Inside Blood analysis of this article appears in the frontof this issue.

Reprints: Deborah Thomas, Department of Leukemia, The University of Texas M. D. Anderson Cancer Center, 1515 Holcombe Blvd, Unit 428, Houston, TX 77030; e-mail: debthomas{at}mdanderson.org.

   References

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Abstract
Introduction
Patients and methods
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Discussion
References

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  Copyright © 2004 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2004 by American Society of Hematology Online ISSN: 1528-0020