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Korean J Hematol 2011; 46(3):

Published online September 30, 2011

https://doi.org/10.5045/kjh.2011.46.3.169

© The Korean Society of Hematology

Recent advances in the path toward the cure for chronic myeloid leukemia

Dong-Wook Kim*

Department of Hematology, Seoul St. Mary's Hospital, The Catholic University of Korea, Seoul, Korea.

Correspondence to : Correspondence to Department of Hematology, Seoul St. Mary's Hospital, The Catholic University of Korea, 505 Banpo-dong, Seocho-gu, Seoul 137-701, Korea. Tel: +82-2-2258-7030, Fax: +82-2-593-2522, dwkim@catholic.ac.kr

Received: September 1, 2011; Accepted: September 9, 2011

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Through the phase 3 International Randomized Study of Interferon vs. STI571 (IRIS) trial, imatinib emerged as the standard treatment for chronic myeloid leukemia (CML) and has successfully prolonged the duration of both the chronic phase (CP) and the disease-free state. The majority of newly diagnosed patients treated for CP-CML achieve a complete cytogenetic response (CCyR), and over time, most of these eventually achieve major molecular responses (MMRs) and even complete molecular responses (CMRs). In ongoing phase 3 randomized trials of second-generation tyrosine kinase inhibitors (TKIs), nilotinib and dasatinib have been found to have superior efficacies in helping achieve cytogenetic and molecular responses, including MMRs and CMRs. However, only the MMR rate was significantly higher in bosutinib compared with the imatinib control, but not in CCyR rate. Current reports of imatinib discontinuation suggested that achieving CMR is an important prerequisite for CML to be cured. Recent data from the STIM (Stop Imatinib) trial showed that imatinib can be successfully discontinued in patients who achieve a certain level of CMR. Standardized real-time quantitative reverse transcriptase-polymerase chain reaction (RQ-PCR) assays have been available in routine clinical practice, and efforts are being focused on achieving higher sensitivity and optimizing the time of imatinib discontinuation. Although very few patients are cured by administration of only Bcr-Abl TKIs, including imatinib and second-generation TKIs, current advances may eventually make this possible. This report summarizes the detailed clinical data obtained in the DASISION, ENESTnd, and BELA studies and discusses high-sensitivity detection methods and future therapeutic strategies.

Keywords CML, Imatinib, Nilotinib, Dasatinib, PCR, Leukemia stem cell

1. Incidence of molecular responses

In the IRIS trial, previously untreated CP-CML patients (N=1,106) were randomly assigned to receive either imatinib (N=553) or interferon (IFN)-α plus cytarabine (N=553). During the sixth year of study treatment, the cumulative best CCyR rate was 82%. The estimated event-free survival at 6 years was 83%, and the estimated progression-free survival (PFS) rate was 93% [1]. The IRIS study showed that during the median follow-up of 19 months, 21% and 4% of patients in the imatinib group had achieved MMR and CMR, respectively [2]. In a substudy of 53 imatinib-treated IRIS patients, the probability of Bcr-Abl being undetectable increased considerably from 36 to 81 months of first-line imatinib treatment (7% vs. 52%). Bcr-Abl became undetectable in 18 of 53 patients, and none of whom lost MMR after a median follow-up of 33 months. In contrast, MMR was lost in 6 of 22 (27%) patients with sustained detectable Bcr-Abl [3]. In a study conducted in the Hammersmith hospital on 204 CP-CML patients receiving imatinib as first-line therapy, at 5 years, 159 patients (77%) had achieved a CCyR (median time, 7 months; range, 3-55.4 months), 80 (39%) had achieved an MMR (median time, 15.7 months; range, 2-73 months), and 10 (5%) had achieved a CMR (median time, 30.7 months; range, 12-67.4 months). The cumulative incidences of CCyR and MMR were 82.7% and 50.1%, respectively. Of the 80 patients who achieved an MMR, the response was sustained in 90% [4]. In our current study with 363 new CP patients, the cumulative incidences of CCyR, MMR, and CMR4.5 at 5 years increased to 92%, 52%, and 11%, respectively. At 7 years, the cumulative incidences of CCyR, MMR, and CMR4.5 were 94%, 60%, and 14% respectively. In addition, when compared to the group receiving less than 400 mg/d, the 400 mg/d group demonstrated a better 6-year cumulative incidence of MMR (82% vs. 66%, respectively, P=0.014) and CMR4.5 (38% vs. 13%, respectively, P=0.0042) (unpublished data). Therefore, response rates might be directly correlated with treatment intensity.

2. Significance of molecular responses

Several studies have reported different clinical implications of MMRs at specific time points in long-term survival outcomes. The IRIS study proved that MMRs at 12 and 18 months can predict significantly better PFS [2]. Moreover, the achievement of an MMR by 18 months of therapy was proposed to be the goal of therapy [5]. However, other studies have reported that such differences may not be clinically relevant and that only the achievement of CCyR was significant in order to predict survival [4, 6]. Early achievement of molecular responses correlates with achievement of MMRs and a reduction in the number of events. As summarized in Table 1, the prognostic significance of early molecular responses is clear; patients with a Bcr-Abl ratio of 1% or less at 3 months had very low event rates, with a median follow-up of 53 months [7]. The CMR rate gradually increased with continuing imatinib treatment, and CMR was more common in patients who achieved an MMR early.

1. Frontline second-generation TKI studies; ENESTnd, DASISION, and BELA

Investigations are currently underway to determine the efficacy and safety of second-generation Bcr-Abl TKIs in the treatment of newly diagnosed CP-CML, including the multicenter, phase 3, randomized clinical trials "Evaluating Nilotinib Efficacy and Safety in Clinical Trials-Newly Diagnosed Patients" (ENESTnd) [8] and "Dasatinib versus Imatinib Study in Treatment-Naïve CML Patients" (DASISION) [9]. These studies have shown that Nilotinib and dasatinib have superior efficacies than imatinib. Bosutinib, currently an investigational agent not yet approved for CML treatment, is also being studied in the "Bosutinib versus Imatinib in Patients with Chronic Phase Chronic Myeloid Leukemia" (BELA) trial [10]. In the ENESTnd study, 846 patients were randomly assigned to receive 300 mg nilotinib twice daily (N=282), 400 mg nilotinib twice daily (N=281), and 400 mg imatinib once daily (QD; N=283). In the DASISION trial, 519 patients with newly diagnosed CP-CML were randomized to receive first-line treatment with either 100 mg dasatinib QD (N=259) or 400 mg imatinib QD (N=260). In the BELA study, 502 patients with newly diagnosed CP-CML were randomized to receive first-line treatment with either 500 mg bosutinib QD (N=250) or 400 mg imatinib QD (N=252). The ENESTnd, DASISION, and BELA trials had different study designs, primary end-points, and definitions. Therefore, direct comparison of the results is not possible. Presently, 24 months of data from the ENESTnd and DASISION studies, and 18 months of data from the BELA study are available, and significantly higher rates of MMR and CMR4.5 were observed with nilotinib, dasatinib, and bosutinib than with imatinib [10-12].

2. Comparison of molecular responses between second-generation TKIs and Imatinib

By 24 months into the ENESTnd study, significantly more patients had achieved an MMR with nilotinib than with imatinib: 71% of patients receiving nilotinib at 300 mg twice daily, 67% of patients receiving nilotinib at 400 mg twice daily, and 44% of patients receiving imatinib showed an MMR (P<0.0001 for both comparisons). In addition, significantly more patients in the nilotinib groups achieved a CMR4.5 at any time than those in the imatinib group (26% of patients receiving nilotinib at 300 mg twice daily, 21% of patients receiving nilotinib at 400 mg twice daily, and 10% of patients receiving imatinib achieved a CMR) [11]. By 24 months into the DASISON study, the rate of MMRs was superior for dasatinib vs. imatinib (64% vs. 46%, respectively), and the CMR4.5 rate was also higher for dasatinib vs. imatinib (17% vs. 8%, respectively) [12]. From 12 to 24 months, dasatinib also continued to show better efficacy than imatinib for the treatment of CML. The MMR rate at 18 months in the BELA study was higher with bosutinib (46%; 95% CI, 39-52%) than with imatinib (38%; 95% CI, 32-44%), and 9% of patients achieved a CMR4.5 with bosutinib, compared with 4% who achieved a CMR with imatinib [10]. Overall, patients achieved their first molecular responses faster and deeper with all 3 of these second-generation TKIs than with imatinib.

1. Discontinuation of imatinib

Although imatinib therapy is effective and currently considered a front-line therapy in patients with CML, it is still unclear whether intermittent imatinib therapy can be safely employed in particular situations such as pregnancy and serious adverse events. Thus far, in studies on the discontinuation of TKI therapy, 100% of patients with less than a CMR have relapsed (Table 2) [13-15]. Therefore, it may be necessary for patients to achieve a CMR before physicians consider potentially discontinuing TKI therapy [16]. In our study, the majority of patients maintained their best achieved response after resuming imatinib treatment [13]. Therefore, although imatinib cannot be discontinued completely, transient interruption can be considered for the treatment of patients with CML in particular situations such as serious or life-threatening concomitant diseases, pregnancy, or major surgery.

In the STIM study, patients with more than 2 years of documented CMRs while on imatinib therapy attempted therapy discontinuation. A total of 69 patients were followed up for more than 12 months. Nineteen of 34 patients (55.9%) who received prior INF-α therapy relapsed, and 23 of 35 patients (65.7%) who received imatinib as first-line therapy relapsed. The Sokal scores showed that 17 of 35 patients (48.6%), 15 of 23 patients (65.2%), and 7 of 8 patients (87.5%) who relapsed were at low, intermediate, or high risk, respectively. In addition, 27 of 51 patients (52.9%) who received more than 50 months of imatinib treatment relapsed, compared with 15 of 18 patients (83.3%) who received less than 50 months of imatinib therapy [16]. Typically, patients who enrolled in the STIM trial had deeper and longer molecular responses while on imatinib therapy than patients in other studies, and therefore, discontinuation of therapy should not be attempted outside of a controlled clinical trial with frequent monitoring.

2. Discontinuation of second-generation TKIs

In a study on discontinuation of dasatinib or nilotinib in 17 adult patients who had achieved a CMR4.5 [17], of the 12 patients with a minimum follow-up period of 6 months (median, 12; range, 7-18), 11 had imatinib intolerance and 1 had imatinib resistance, and 30% (4/12) of patients lost the MMR by 6 months of discontinuation. The MMR was rapidly regained upon re-introduction of early second-generation TKIs. Treatment was also restarted in 1 patient in whom there was no MMR loss but who showed CMR loss on 2 consecutive assessments. Seven patients remained off therapy at the last follow-up after a median of 11 months (range, 7-18), with either a stable CMR or weakly detectable Bcr-Abl transcripts on one or more occasions. Although a longer follow-up with more patients will be required, the study provided a basis for further studies on discontinuation of second-generation TKIs. In addition, since current frontline second-generation TKI data from the DASISION and ENESTnd studies are showing that the probability of persistent CMR by 36 months of follow-up remains higher with dasatinib and nilotinib than with imatinib, more patients receiving second-generation TKI therapies may be safely discontinued in the future.

1. Definition of molecular responses by conventional RQ-PCR

The principal means of monitoring a patient's response to therapy is to assess their hematologic, cytogenetic, and molecular responses as well as their long-term outcomes [5, 18]. Since therapies for CML have improved, patients have been able to achieve responses at the molecular level. Therefore, more sensitive measurements are necessary to detect minimal residual disease (MRD). Real-time quantitative polymerase chain reaction (RQ-PCR) assessment can detect deeper levels of response, up to a 5-log reduction [6]. Generally, molecular response is a measure of the level of Bcr-Abl transcripts as determined by RQ-PCR and is described as a ratio of Bcr-Abl to a housekeeping gene (such as ABL, BCR, or GUS). An MMR is achieved when a patient reaches a 3-log reduction in Bcr-Abl transcripts from a baseline value defined in the IRIS trial [2, 19]. Since inter-laboratory variation in the methods of conducting RQ-PCR makes comparison of data between laboratories difficult, the international scale (IS) has been developed to allow for cross-laboratory comparison of PCR results [20]. The IS is defined by 2 values: (1) a baseline value (i.e., pretreatment with imatinib) of the Bcr-Abl/ABL ratio, which was defined based on an analysis of baseline levels in patients from the IRIS trial (100%), and (2) a 3-log reduction thereof, or a reduction to 0.1% or less, which is defined as an MMR [2]. To convert the PCR results obtained in a laboratory to the IS, the results are modified using a laboratory-specific conversion factor that is calculated by comparing patient samples against a reference method [20]. Deeper molecular responses are now defined as achieving a CMR4.0 of more than 4.0-log reduction (Bcr-AblIS≤0.01%), a CMR4.5 of more than 4.5-log reduction (Bcr-AblIS≤0.005%), and a CMR5.0 of more than 5-log reduction in Bcr-Abl transcripts (Bcr-AblIS≤0.001%) [21, 22]. In the STIM trial, the selection criteria for candidates was based on the duration of imatinib therapy and the duration of PCR negativity prior to discontinuation, and conventional RQ-PCR was employed to measure PCR negativity. However, the fact that the absolute number of residual leukemia clones could not be measured under the detection limits of conventional RQ-PCR might have resulted in relapse in more than half of the patients. This indicates that conclusions cannot be drawn about whether a patient could safely discontinue therapy solely based on conventional RQ-PCR. The absence of Bcr-Abl transcripts in conventional RQ-PCR is sometimes unreliable since some patients, despite being PCR-negative, relapse and PCR negativity may be maintained after imatinib discontinuation [23, 24]. It might be necessary to develop more sensitive assays that can provide a more reliable estimation of the therapeutic response of the patient, and thus allow further classification of patients who may discontinue imatinib without the risk of relapse. With the advent of more potent TKIs, more sensitive assays would also be able to extend the period of measurable disease by several years in most patients with CML. This will help in further assessment of the kinetics of Bcr-Abl under the detection limit of conventional RQ-PCR, whereas conventional RQ-PCR will become less useful for many patients who show dramatic responses to therapy and in whom Bcr-Abl transcripts in undetectable.

2. High-sensitivity PCR technologies

With the emergence of increasingly efficacious therapies leading up to imatinib, the majority of patients with Ph+ CML were able to achieve deeper levels of response. Increasingly sophisticated and sensitive methods of disease detection have been developed in parallel to facilitate the detection of these deeper patient responses. To demonstrate the feasibility of more sensitive approaches, several methods have been developed using DNA-based PCR [25] and RNA-based PCR assays [26]. Replicated PCR (rRQ-PCR), DNA-based PCR, and RNA-based digital PCR (dPCR) assays have successfully detected Bcr-Abl transcripts that were previously not detectable by conventional RQ-PCR, and these data show the potential feasibility of high-sensitivity PCR approaches for molecular monitoring and their clinical relevance in future strategies for drug discontinuation by allowing further characterization of patients who achieve PCR negativity in conventional RQ-PCR assays. In our study, rRQ-PCR allowed for a 2-log improvement in detection sensitivity, and therefore, use of this method might increase the chances of detecting very low Bcr-Abl transcript levels, the probability of which increases with the number of repetitions [26]. In addition to rRQ-PCR, the concept of partitioning in dPCR, in conjunction with a pre-amplification step, also successfully achieved a 2-3-log improvement in detection sensitivity. Although implementation of a pre-amplification step prior to conventional RQ-PCR also increased the sensitivity to a level comparable to that of rRQ-PCR, significant variations in the detection of Bcr-Abl copy numbers were evident in samples with low levels of Bcr-Abl transcripts in replicate experiments. Therefore, although the sensitivity was improved by pre-amplification in conventional RQ-PCR, dPCR would be an attractive alternative tool for accurate detection of low levels of MRD with high sensitivity. In the future, more strict PCR sensitivity criteria using highly sensitive technologies should be employed to accurately assess Bcr-Abl transcript levels prior to discontinuation and then to consider whether discontinuation of TKI therapy may be safe.

1. Definition of curability

In practical terms, some criteria have defined curability as (1) sustained molecular response, (2) successful discontinuation of TKI therapy, (3) 100% CML-related survival, and (4) quality of life (QoL) comparable to that of age-matched population. Although considerable progress has recently been made in CML therapy, a true cure for the disease can only be obtained by our present therapeutic means in a rather small minority of patients. Since leukemia stem cells (LSCs) in CML are insensitive to imatinib treatment [27], and the self-renewal ability of LSCs can result in re-emergence of disease even after a long period of RQ-PCR negativity, sustained undetectable MRD is obtained only in a minority of CML patients treated with TKIs. It still is not clear whether these patients are definitively cured of leukemia, or whether LSCs persist in their bone marrow. The relationship between LSC persistence and the potential risk of disease relapse for patients with long-term undetectable MRD warrants further investigation [28].

2. New therapeutic targets for curing CML

Although the molecular differences in Bcr-Abl expression between hematopoietic stem cells (HSCs) and LSCs are still unclear, the best means of identifying stem cell targets in CML is to fully understand CML-initiating genetic changes. Recently, several new targets or drugs have been found to inhibit LSCs in cultured human CD34+ CML cells or in mouse models of Bcr-Abl-induced CML, including an Alox5 pathway inhibitor, Hsp90 inhibitors, omacetaxine, a hedgehog inhibitor, and the farnesyl transferase inhibitor BMS-214662. To obtain the ultimate goal of a cure for CML, 2 strategies have been tested. One important strategy has been to inhibit target genes such as those encoding hedgehog [29], Wnt/β-catenin [30], and Bim-1 [31] in order to functionally regulate both normal stem cells and LSCs. Another approach has been the specific targeting of LSC-related genes, but not those of normal stem cells, for developing new anticancer therapies in the future (Fig. 1) [32].

Currently, several drugs targeting LSCs have been reported. The hedgehog pathway is active in many tissues, where it plays a critical role in hematopoiesis and is activated in Ph+ CML stem cells [33]. The smoothened antagonist, LDE225, is currently in phase 1 clinical trial for the treatment of Ph+ CML and other cancers. Janus kinase 2 inhibition may inhibit stem cells [34], and INF may stimulate quiescent LSCs to proliferate, making them susceptible to TKI therapy [35]. Residual disease may be the result of the presence of LSCs, which can act as a reservoir of disease that cannot be eradicated by TKI therapy alone [27, 36]. Relapses can occur even in patients who have undergone potentially curative stem cell transplants, suggesting that residual disease may be present even in patients with prolonged CMRs [37, 38]. Therefore, the inhibition of LSCs may be a crucial step in curing CML. Several trials utilizing INF maintenance therapies and/or combination therapies with potent TKIs and/or LSC-targeting agents are ongoing. Future CML management might include earlier use of these agents to help more patients achieve CMRs and may be a means of curing CML.

During the past decade, considerable progress has been made in understanding the biology of CML, which has raised hopes that this disease may be curable. Early intensification using combination therapies with more potent TKI- and LSC-targeted agents is required for the development of more sensitive PCR assays. The achievement of deeper responses, measured only by highly sensitive assays, will establish a necessary first step toward potentially discontinuing drug therapy.

Table. 1.

Table 1 Relationship between early molecular response and patient outcomes.

a)Event was defined as loss of complete hematologic response, loss of major cytogenetic response, or an increasing white cell count (definedas a doubling of the count to more than 20×109/L on 2 occasions at least 1 month apart), progression to accelerated phase/blast crisis, or death from any cause during imatinib treatment.

Abbreviation: MMR, major molecular response.


Table. 2.

Table 2 Results of imatinib discontinuation in different clinical settings.

Abbreviations: CCyR, complete cytogenetic response; MMR, major molecular response; CMR, complete molecular response.


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Article

Review Article

Korean J Hematol 2011; 46(3): 169-174

Published online September 30, 2011 https://doi.org/10.5045/kjh.2011.46.3.169

Copyright © The Korean Society of Hematology.

Recent advances in the path toward the cure for chronic myeloid leukemia

Dong-Wook Kim*

Department of Hematology, Seoul St. Mary's Hospital, The Catholic University of Korea, Seoul, Korea.

Correspondence to: Correspondence to Department of Hematology, Seoul St. Mary's Hospital, The Catholic University of Korea, 505 Banpo-dong, Seocho-gu, Seoul 137-701, Korea. Tel: +82-2-2258-7030, Fax: +82-2-593-2522, dwkim@catholic.ac.kr

Received: September 1, 2011; Accepted: September 9, 2011

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract

Through the phase 3 International Randomized Study of Interferon vs. STI571 (IRIS) trial, imatinib emerged as the standard treatment for chronic myeloid leukemia (CML) and has successfully prolonged the duration of both the chronic phase (CP) and the disease-free state. The majority of newly diagnosed patients treated for CP-CML achieve a complete cytogenetic response (CCyR), and over time, most of these eventually achieve major molecular responses (MMRs) and even complete molecular responses (CMRs). In ongoing phase 3 randomized trials of second-generation tyrosine kinase inhibitors (TKIs), nilotinib and dasatinib have been found to have superior efficacies in helping achieve cytogenetic and molecular responses, including MMRs and CMRs. However, only the MMR rate was significantly higher in bosutinib compared with the imatinib control, but not in CCyR rate. Current reports of imatinib discontinuation suggested that achieving CMR is an important prerequisite for CML to be cured. Recent data from the STIM (Stop Imatinib) trial showed that imatinib can be successfully discontinued in patients who achieve a certain level of CMR. Standardized real-time quantitative reverse transcriptase-polymerase chain reaction (RQ-PCR) assays have been available in routine clinical practice, and efforts are being focused on achieving higher sensitivity and optimizing the time of imatinib discontinuation. Although very few patients are cured by administration of only Bcr-Abl TKIs, including imatinib and second-generation TKIs, current advances may eventually make this possible. This report summarizes the detailed clinical data obtained in the DASISION, ENESTnd, and BELA studies and discusses high-sensitivity detection methods and future therapeutic strategies.

Keywords: CML, Imatinib, Nilotinib, Dasatinib, PCR, Leukemia stem cell

LONG-TERM MOLECULAR RESPONSE OF IMATINIB: DATA FROM IRIS AND HAMMERSMITH AND SEOUL ST. MARY'S HOSPITAL

1. Incidence of molecular responses

In the IRIS trial, previously untreated CP-CML patients (N=1,106) were randomly assigned to receive either imatinib (N=553) or interferon (IFN)-α plus cytarabine (N=553). During the sixth year of study treatment, the cumulative best CCyR rate was 82%. The estimated event-free survival at 6 years was 83%, and the estimated progression-free survival (PFS) rate was 93% [1]. The IRIS study showed that during the median follow-up of 19 months, 21% and 4% of patients in the imatinib group had achieved MMR and CMR, respectively [2]. In a substudy of 53 imatinib-treated IRIS patients, the probability of Bcr-Abl being undetectable increased considerably from 36 to 81 months of first-line imatinib treatment (7% vs. 52%). Bcr-Abl became undetectable in 18 of 53 patients, and none of whom lost MMR after a median follow-up of 33 months. In contrast, MMR was lost in 6 of 22 (27%) patients with sustained detectable Bcr-Abl [3]. In a study conducted in the Hammersmith hospital on 204 CP-CML patients receiving imatinib as first-line therapy, at 5 years, 159 patients (77%) had achieved a CCyR (median time, 7 months; range, 3-55.4 months), 80 (39%) had achieved an MMR (median time, 15.7 months; range, 2-73 months), and 10 (5%) had achieved a CMR (median time, 30.7 months; range, 12-67.4 months). The cumulative incidences of CCyR and MMR were 82.7% and 50.1%, respectively. Of the 80 patients who achieved an MMR, the response was sustained in 90% [4]. In our current study with 363 new CP patients, the cumulative incidences of CCyR, MMR, and CMR4.5 at 5 years increased to 92%, 52%, and 11%, respectively. At 7 years, the cumulative incidences of CCyR, MMR, and CMR4.5 were 94%, 60%, and 14% respectively. In addition, when compared to the group receiving less than 400 mg/d, the 400 mg/d group demonstrated a better 6-year cumulative incidence of MMR (82% vs. 66%, respectively, P=0.014) and CMR4.5 (38% vs. 13%, respectively, P=0.0042) (unpublished data). Therefore, response rates might be directly correlated with treatment intensity.

2. Significance of molecular responses

Several studies have reported different clinical implications of MMRs at specific time points in long-term survival outcomes. The IRIS study proved that MMRs at 12 and 18 months can predict significantly better PFS [2]. Moreover, the achievement of an MMR by 18 months of therapy was proposed to be the goal of therapy [5]. However, other studies have reported that such differences may not be clinically relevant and that only the achievement of CCyR was significant in order to predict survival [4, 6]. Early achievement of molecular responses correlates with achievement of MMRs and a reduction in the number of events. As summarized in Table 1, the prognostic significance of early molecular responses is clear; patients with a Bcr-Abl ratio of 1% or less at 3 months had very low event rates, with a median follow-up of 53 months [7]. The CMR rate gradually increased with continuing imatinib treatment, and CMR was more common in patients who achieved an MMR early.

MOLECULAR RESPONSES IN ENESTnd, DASISION, AND BELA TRIALS

1. Frontline second-generation TKI studies; ENESTnd, DASISION, and BELA

Investigations are currently underway to determine the efficacy and safety of second-generation Bcr-Abl TKIs in the treatment of newly diagnosed CP-CML, including the multicenter, phase 3, randomized clinical trials "Evaluating Nilotinib Efficacy and Safety in Clinical Trials-Newly Diagnosed Patients" (ENESTnd) [8] and "Dasatinib versus Imatinib Study in Treatment-Naïve CML Patients" (DASISION) [9]. These studies have shown that Nilotinib and dasatinib have superior efficacies than imatinib. Bosutinib, currently an investigational agent not yet approved for CML treatment, is also being studied in the "Bosutinib versus Imatinib in Patients with Chronic Phase Chronic Myeloid Leukemia" (BELA) trial [10]. In the ENESTnd study, 846 patients were randomly assigned to receive 300 mg nilotinib twice daily (N=282), 400 mg nilotinib twice daily (N=281), and 400 mg imatinib once daily (QD; N=283). In the DASISION trial, 519 patients with newly diagnosed CP-CML were randomized to receive first-line treatment with either 100 mg dasatinib QD (N=259) or 400 mg imatinib QD (N=260). In the BELA study, 502 patients with newly diagnosed CP-CML were randomized to receive first-line treatment with either 500 mg bosutinib QD (N=250) or 400 mg imatinib QD (N=252). The ENESTnd, DASISION, and BELA trials had different study designs, primary end-points, and definitions. Therefore, direct comparison of the results is not possible. Presently, 24 months of data from the ENESTnd and DASISION studies, and 18 months of data from the BELA study are available, and significantly higher rates of MMR and CMR4.5 were observed with nilotinib, dasatinib, and bosutinib than with imatinib [10-12].

2. Comparison of molecular responses between second-generation TKIs and Imatinib

By 24 months into the ENESTnd study, significantly more patients had achieved an MMR with nilotinib than with imatinib: 71% of patients receiving nilotinib at 300 mg twice daily, 67% of patients receiving nilotinib at 400 mg twice daily, and 44% of patients receiving imatinib showed an MMR (P<0.0001 for both comparisons). In addition, significantly more patients in the nilotinib groups achieved a CMR4.5 at any time than those in the imatinib group (26% of patients receiving nilotinib at 300 mg twice daily, 21% of patients receiving nilotinib at 400 mg twice daily, and 10% of patients receiving imatinib achieved a CMR) [11]. By 24 months into the DASISON study, the rate of MMRs was superior for dasatinib vs. imatinib (64% vs. 46%, respectively), and the CMR4.5 rate was also higher for dasatinib vs. imatinib (17% vs. 8%, respectively) [12]. From 12 to 24 months, dasatinib also continued to show better efficacy than imatinib for the treatment of CML. The MMR rate at 18 months in the BELA study was higher with bosutinib (46%; 95% CI, 39-52%) than with imatinib (38%; 95% CI, 32-44%), and 9% of patients achieved a CMR4.5 with bosutinib, compared with 4% who achieved a CMR with imatinib [10]. Overall, patients achieved their first molecular responses faster and deeper with all 3 of these second-generation TKIs than with imatinib.

STUDIES ON DISCONTINUATION OF TKIs

1. Discontinuation of imatinib

Although imatinib therapy is effective and currently considered a front-line therapy in patients with CML, it is still unclear whether intermittent imatinib therapy can be safely employed in particular situations such as pregnancy and serious adverse events. Thus far, in studies on the discontinuation of TKI therapy, 100% of patients with less than a CMR have relapsed (Table 2) [13-15]. Therefore, it may be necessary for patients to achieve a CMR before physicians consider potentially discontinuing TKI therapy [16]. In our study, the majority of patients maintained their best achieved response after resuming imatinib treatment [13]. Therefore, although imatinib cannot be discontinued completely, transient interruption can be considered for the treatment of patients with CML in particular situations such as serious or life-threatening concomitant diseases, pregnancy, or major surgery.

In the STIM study, patients with more than 2 years of documented CMRs while on imatinib therapy attempted therapy discontinuation. A total of 69 patients were followed up for more than 12 months. Nineteen of 34 patients (55.9%) who received prior INF-α therapy relapsed, and 23 of 35 patients (65.7%) who received imatinib as first-line therapy relapsed. The Sokal scores showed that 17 of 35 patients (48.6%), 15 of 23 patients (65.2%), and 7 of 8 patients (87.5%) who relapsed were at low, intermediate, or high risk, respectively. In addition, 27 of 51 patients (52.9%) who received more than 50 months of imatinib treatment relapsed, compared with 15 of 18 patients (83.3%) who received less than 50 months of imatinib therapy [16]. Typically, patients who enrolled in the STIM trial had deeper and longer molecular responses while on imatinib therapy than patients in other studies, and therefore, discontinuation of therapy should not be attempted outside of a controlled clinical trial with frequent monitoring.

2. Discontinuation of second-generation TKIs

In a study on discontinuation of dasatinib or nilotinib in 17 adult patients who had achieved a CMR4.5 [17], of the 12 patients with a minimum follow-up period of 6 months (median, 12; range, 7-18), 11 had imatinib intolerance and 1 had imatinib resistance, and 30% (4/12) of patients lost the MMR by 6 months of discontinuation. The MMR was rapidly regained upon re-introduction of early second-generation TKIs. Treatment was also restarted in 1 patient in whom there was no MMR loss but who showed CMR loss on 2 consecutive assessments. Seven patients remained off therapy at the last follow-up after a median of 11 months (range, 7-18), with either a stable CMR or weakly detectable Bcr-Abl transcripts on one or more occasions. Although a longer follow-up with more patients will be required, the study provided a basis for further studies on discontinuation of second-generation TKIs. In addition, since current frontline second-generation TKI data from the DASISION and ENESTnd studies are showing that the probability of persistent CMR by 36 months of follow-up remains higher with dasatinib and nilotinib than with imatinib, more patients receiving second-generation TKI therapies may be safely discontinued in the future.

HIGH-SENSITIVITY PCR TECHNOLOGY

1. Definition of molecular responses by conventional RQ-PCR

The principal means of monitoring a patient's response to therapy is to assess their hematologic, cytogenetic, and molecular responses as well as their long-term outcomes [5, 18]. Since therapies for CML have improved, patients have been able to achieve responses at the molecular level. Therefore, more sensitive measurements are necessary to detect minimal residual disease (MRD). Real-time quantitative polymerase chain reaction (RQ-PCR) assessment can detect deeper levels of response, up to a 5-log reduction [6]. Generally, molecular response is a measure of the level of Bcr-Abl transcripts as determined by RQ-PCR and is described as a ratio of Bcr-Abl to a housekeeping gene (such as ABL, BCR, or GUS). An MMR is achieved when a patient reaches a 3-log reduction in Bcr-Abl transcripts from a baseline value defined in the IRIS trial [2, 19]. Since inter-laboratory variation in the methods of conducting RQ-PCR makes comparison of data between laboratories difficult, the international scale (IS) has been developed to allow for cross-laboratory comparison of PCR results [20]. The IS is defined by 2 values: (1) a baseline value (i.e., pretreatment with imatinib) of the Bcr-Abl/ABL ratio, which was defined based on an analysis of baseline levels in patients from the IRIS trial (100%), and (2) a 3-log reduction thereof, or a reduction to 0.1% or less, which is defined as an MMR [2]. To convert the PCR results obtained in a laboratory to the IS, the results are modified using a laboratory-specific conversion factor that is calculated by comparing patient samples against a reference method [20]. Deeper molecular responses are now defined as achieving a CMR4.0 of more than 4.0-log reduction (Bcr-AblIS≤0.01%), a CMR4.5 of more than 4.5-log reduction (Bcr-AblIS≤0.005%), and a CMR5.0 of more than 5-log reduction in Bcr-Abl transcripts (Bcr-AblIS≤0.001%) [21, 22]. In the STIM trial, the selection criteria for candidates was based on the duration of imatinib therapy and the duration of PCR negativity prior to discontinuation, and conventional RQ-PCR was employed to measure PCR negativity. However, the fact that the absolute number of residual leukemia clones could not be measured under the detection limits of conventional RQ-PCR might have resulted in relapse in more than half of the patients. This indicates that conclusions cannot be drawn about whether a patient could safely discontinue therapy solely based on conventional RQ-PCR. The absence of Bcr-Abl transcripts in conventional RQ-PCR is sometimes unreliable since some patients, despite being PCR-negative, relapse and PCR negativity may be maintained after imatinib discontinuation [23, 24]. It might be necessary to develop more sensitive assays that can provide a more reliable estimation of the therapeutic response of the patient, and thus allow further classification of patients who may discontinue imatinib without the risk of relapse. With the advent of more potent TKIs, more sensitive assays would also be able to extend the period of measurable disease by several years in most patients with CML. This will help in further assessment of the kinetics of Bcr-Abl under the detection limit of conventional RQ-PCR, whereas conventional RQ-PCR will become less useful for many patients who show dramatic responses to therapy and in whom Bcr-Abl transcripts in undetectable.

2. High-sensitivity PCR technologies

With the emergence of increasingly efficacious therapies leading up to imatinib, the majority of patients with Ph+ CML were able to achieve deeper levels of response. Increasingly sophisticated and sensitive methods of disease detection have been developed in parallel to facilitate the detection of these deeper patient responses. To demonstrate the feasibility of more sensitive approaches, several methods have been developed using DNA-based PCR [25] and RNA-based PCR assays [26]. Replicated PCR (rRQ-PCR), DNA-based PCR, and RNA-based digital PCR (dPCR) assays have successfully detected Bcr-Abl transcripts that were previously not detectable by conventional RQ-PCR, and these data show the potential feasibility of high-sensitivity PCR approaches for molecular monitoring and their clinical relevance in future strategies for drug discontinuation by allowing further characterization of patients who achieve PCR negativity in conventional RQ-PCR assays. In our study, rRQ-PCR allowed for a 2-log improvement in detection sensitivity, and therefore, use of this method might increase the chances of detecting very low Bcr-Abl transcript levels, the probability of which increases with the number of repetitions [26]. In addition to rRQ-PCR, the concept of partitioning in dPCR, in conjunction with a pre-amplification step, also successfully achieved a 2-3-log improvement in detection sensitivity. Although implementation of a pre-amplification step prior to conventional RQ-PCR also increased the sensitivity to a level comparable to that of rRQ-PCR, significant variations in the detection of Bcr-Abl copy numbers were evident in samples with low levels of Bcr-Abl transcripts in replicate experiments. Therefore, although the sensitivity was improved by pre-amplification in conventional RQ-PCR, dPCR would be an attractive alternative tool for accurate detection of low levels of MRD with high sensitivity. In the future, more strict PCR sensitivity criteria using highly sensitive technologies should be employed to accurately assess Bcr-Abl transcript levels prior to discontinuation and then to consider whether discontinuation of TKI therapy may be safe.

THERAPEUTIC STRATEGIES FOR POTENTIAL CURE

1. Definition of curability

In practical terms, some criteria have defined curability as (1) sustained molecular response, (2) successful discontinuation of TKI therapy, (3) 100% CML-related survival, and (4) quality of life (QoL) comparable to that of age-matched population. Although considerable progress has recently been made in CML therapy, a true cure for the disease can only be obtained by our present therapeutic means in a rather small minority of patients. Since leukemia stem cells (LSCs) in CML are insensitive to imatinib treatment [27], and the self-renewal ability of LSCs can result in re-emergence of disease even after a long period of RQ-PCR negativity, sustained undetectable MRD is obtained only in a minority of CML patients treated with TKIs. It still is not clear whether these patients are definitively cured of leukemia, or whether LSCs persist in their bone marrow. The relationship between LSC persistence and the potential risk of disease relapse for patients with long-term undetectable MRD warrants further investigation [28].

2. New therapeutic targets for curing CML

Although the molecular differences in Bcr-Abl expression between hematopoietic stem cells (HSCs) and LSCs are still unclear, the best means of identifying stem cell targets in CML is to fully understand CML-initiating genetic changes. Recently, several new targets or drugs have been found to inhibit LSCs in cultured human CD34+ CML cells or in mouse models of Bcr-Abl-induced CML, including an Alox5 pathway inhibitor, Hsp90 inhibitors, omacetaxine, a hedgehog inhibitor, and the farnesyl transferase inhibitor BMS-214662. To obtain the ultimate goal of a cure for CML, 2 strategies have been tested. One important strategy has been to inhibit target genes such as those encoding hedgehog [29], Wnt/β-catenin [30], and Bim-1 [31] in order to functionally regulate both normal stem cells and LSCs. Another approach has been the specific targeting of LSC-related genes, but not those of normal stem cells, for developing new anticancer therapies in the future (Fig. 1) [32].

Currently, several drugs targeting LSCs have been reported. The hedgehog pathway is active in many tissues, where it plays a critical role in hematopoiesis and is activated in Ph+ CML stem cells [33]. The smoothened antagonist, LDE225, is currently in phase 1 clinical trial for the treatment of Ph+ CML and other cancers. Janus kinase 2 inhibition may inhibit stem cells [34], and INF may stimulate quiescent LSCs to proliferate, making them susceptible to TKI therapy [35]. Residual disease may be the result of the presence of LSCs, which can act as a reservoir of disease that cannot be eradicated by TKI therapy alone [27, 36]. Relapses can occur even in patients who have undergone potentially curative stem cell transplants, suggesting that residual disease may be present even in patients with prolonged CMRs [37, 38]. Therefore, the inhibition of LSCs may be a crucial step in curing CML. Several trials utilizing INF maintenance therapies and/or combination therapies with potent TKIs and/or LSC-targeting agents are ongoing. Future CML management might include earlier use of these agents to help more patients achieve CMRs and may be a means of curing CML.

CONCLUSION

During the past decade, considerable progress has been made in understanding the biology of CML, which has raised hopes that this disease may be curable. Early intensification using combination therapies with more potent TKI- and LSC-targeted agents is required for the development of more sensitive PCR assays. The achievement of deeper responses, measured only by highly sensitive assays, will establish a necessary first step toward potentially discontinuing drug therapy.

Fig 1.

Figure 1.

Role of normal stem cells and leukemia stem cells.

Blood Research 2011; 46: 169-174https://doi.org/10.5045/kjh.2011.46.3.169

Table 1 . Relationship between early molecular response and patient outcomes..

a)Event was defined as loss of complete hematologic response, loss of major cytogenetic response, or an increasing white cell count (definedas a doubling of the count to more than 20×109/L on 2 occasions at least 1 month apart), progression to accelerated phase/blast crisis, or death from any cause during imatinib treatment..

Abbreviation: MMR, major molecular response..


Table 2 . Results of imatinib discontinuation in different clinical settings..

Abbreviations: CCyR, complete cytogenetic response; MMR, major molecular response; CMR, complete molecular response..


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