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Articles

Asparagine levels in the cerebrospinal fluid of children with acute lymphoblastic leukemia treated with pegylated-asparaginase in the induction phase of the AIEOP-BFM ALL 2009 study

Pediatric Hematology-Oncology Unit, Department of Pediatrics, University of Milano-Bicocca, MBBM Foundation, Monza, Italy
Department of Pediatric Hematology and Oncology, University Childrens’ Hospital of Münster, Münster, Germany
Medical Statistics Unit, Department of Clinical Medicine and Prevention, University of Milano-Bicocca, Milan, Italy
Department of Oncology, Laboratory of Cancer Pharmacology, Istituto di Ricerche Farmacologiche Mario Negri IRCCS, Milan, Italy
Department of Oncology, Laboratory of Cancer Pharmacology, Istituto di Ricerche Farmacologiche Mario Negri IRCCS, Milan, Italy
Institute of Biostatistics and Clinical Research, University of Münster, Münster, Germany
Department of Pediatric Hematology and Oncology, University Childrens’ Hospital of Münster, Münster, Germany
Medical Statistics Unit, Department of Clinical Medicine and Prevention, University of Milano-Bicocca, Milan, Italy
Pediatric Hematology-Oncology Unit, Department of Pediatrics, University of Milano-Bicocca, MBBM Foundation, Monza, Italy
Pediatric Hematology-Oncology Unit, Department of Pediatrics, University of Milano-Bicocca, MBBM Foundation, Monza, Italy
Pediatric Hematology-Oncology Unit, Department of Pediatrics, University of Milano-Bicocca, MBBM Foundation, Monza, Italy
Department of Pediatrics, University Medical Center Schleswig-Holstein, Campus Kiel, Kiel, Germany
Department of Pediatrics, University Medical Center Schleswig-Holstein, Campus Kiel, Kiel, Germany
Department of Pediatric Hematology and Oncology, Hannover Medical School, Hannover, Germany
Pediatric Hematology and Oncology, Charité, Berlin, Germany
Pediatric Hematology and Oncology, Hannover Medical School, Hannover, Germany
Children’s Hospital, Augsburg, Germany
Pediatrics 5 (Oncology, Hematology, Immunology); Stuttgart Cancer Center; Klinikum Stuttgart – Olgahospital, Stuttgart, Germany
Department of Pediatric Hematology and Oncology, St. Anna Children’s Hospital, Vienna, Austria
Department of Pediatric Hematology and Oncology, St. Anna Children’s Hospital, Vienna, Austria
Department of Pediatrics and Adolescent Medicine, Medical University of Vienna, Vienna, Austria
Czech Paediatric Haematology/Oncology, Charles University and University Hospital Motol, Prague, Czech Republic
Czech Paediatric Haematology/Oncology, Charles University and University Hospital Motol, Prague, Czech Republic
Department of Pediatric Hemato-Oncology, Ospedale Bambino Gesù, Rome, Italy
Department of Pediatric Hemato-Oncology, Regina Margherita Children’s Hospital, Turin, Italy
Department of Pediatric Hematology-Oncology, Ospedale Pausillipon, Naples, Italy
Department of Pediatric Hematology-Oncology, IRCCS I.G. Gaslini, Genova, Italy
Department of Oncology, Laboratory of Cancer Pharmacology, Istituto di Ricerche Farmacologiche Mario Negri IRCCS, Milan, Italy
Department of Pediatric Hematology and Oncology, University Childrens’ Hospital of Münster, Münster, Germany
Vol. 104 No. 9 (2019): September, 2019 https://doi.org/10.3324/haematol.2018.206433

Abstract

Asparagine levels in cerebrospinal fluid and serum asparaginase activity were monitored in children with acute lymphoblastic leukemia treated with pegylated-asparaginase. The drug was given intravenously at a dose of 2,500 IU/m2 on days 12 and 26. Serum and cerebrospinal fluid samples obtained on days 33 and 45 were analyzed centrally. Since physiological levels of asparagine in the cerebrospinal fluid of children and adolescents are 4-10 μmol/L, in this study asparagine depletion was considered complete when the concentration of asparagine was ≤0.2 μmol/L, i.e. below the lower limit of quantification of the assay used. Over 24 months 736 patients (AIEOP n=245, BFM n=491) and 903 cerebrospinal fluid samples (n=686 on day 33 and n=217 on day 45) were available for analysis. Data were analyzed separately for the AIEOP and BFM cohorts and yielded superimposable results. Independently of serum asparaginase activity levels, cerebrospinal fluid asparagine levels were significantly reduced during the investigated study phase but only 28% of analyzed samples showed complete asparagine depletion while relevant levels, ≥1 μmol/L, were still detectable in around 23% of them. Complete cerebrospinal fluid asparagine depletion was found in around 5-6% and 33-37% of samples at serum asparaginase activity levels <100 and ≥ 1,500 IU/L, respectively. In this study cerebrospinal fluid asparagine levels were reduced during pegylated-asparaginase treatment, but complete depletion was only observed in a minority of patients. No clear threshold of serum pegylated-asparaginase activity level resulting in complete cerebrospinal fluid asparagine depletion was identified. The consistency of the results found in the two independent data sets strengthen the observations of this study. Details of the treatment are available in the European Clinical Trials Database at https://www.clin-icaltrialsregister.eu/ctr-search/trial/2007-004270-43/IT.

Introduction

Asparaginase is one of the major anticancer drugs used in the treatment of acute lymphoblastic leukemia (ALL). The enzyme reduces the levels of asparagine in serum by hydrolyzing it to aspartic acid and ammonia. Currently there are three commercially available asparaginase products.1 The oldest one is the purified native enzyme extracted from Escherichia coli, subsequently also available in a polyethylene glycol conjugated form (PEG-asparaginase) commonly used as the first-line preparation in the treatment of children with ALL throughout Europe and USA. A third asparaginase product derived from Erwinia chrysanthemi (ERW-asparaginase) exists and, due to its structural differences with respect to the E. coli asparaginase products, has been primarily used as a second-line treatment in children with hypersensitivity reactions to the E. coli products.2 Since leukemic cells need exogenous asparagine for their survival much more than the normal host cells do, the depletion of asparagine in serum serves as a surrogate for the anti-leukemic action of asparaginase, no matter which type of product is used. Due to this mechanism of action and to the pharmacodynamic ability of asparaginase products to reduce asparagine pools also in the cerebrospinal fluid (CSF), it has been questioned whether profound and prolonged asparagine depletion, as that determined in the serum, could be of relevance in preventing central nervous system (CNS) relapses.3 Of course, it is exceedingly difficult to ascertain the role of a single drug in the prevention of ALL relapses, especially in an extramedullary compartment such as the CNS where relapses are quite rare. However, in a previous study, patients with higher CSF asparagine levels (>1 μmol/L) during asparaginase treatment were more likely to have isolated CNS relapse.4

Available studies reporting data on CSF asparagine depletion during asparaginase treatment have been mostly performed in limited cohorts of patients and using different asparaginase products, schedules and assays. In the past it has been consistently reported that profound and prolonged CSF asparagine depletion in children treated with standard induction chemotherapy treatment schedules95 is achieved when native forms of asparaginase are used. To this end the conceptual question on how asparaginase products may determine asparagine depletion in the CSF remains unanswered. One possible explanation for the asparagine depletion observed in the CSF could lie in a continuous balance between the serum and CSF asparagine pools.1110 Another possible explanation is that, at peak levels, very small amounts of asparaginase products could cross the blood-brain barrier;12 however, activity levels have never been directly measured in the CSF during the administration of native forms of asparaginase. Given that PEG-asparaginase has a far greater molecular weight than that of the native forms of asparaginase, it is conceivable that it is even more difficult for the pegylated form to cross the blood-brain barrier. Different results have been reported in patients treated with PEG-asparaginase wherein detectable CSF asparagine levels have been almost invariably reported thus suggesting that pharmacodynamic differences exist between the different asparaginase products.15134 We very recently demonstrated, even with the limitations of the experimental preclinical model adopted, that in the CSF of rats asparaginase activity levels could be measured, consistently even if transiently, only for non-pegylated formulations.16

In the international AIEOP-BFM ALL 2009 trial protocol (https://www.clinicaltrialsregister.eu/ctr-search/trial/2007-004270-43/IT), conducted by members of the Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and Berlin-Frankfurt-Münster (BFM) group, children with newly diagnosed ALL have been treated with multiple antileukemic agents, including PEG-asparaginase as the first-line preparation. Since PEG-asparaginase has been used in the AIEOP-BFM ALL 2009 study protocol for the first time as a front-line asparaginase agent instead of the previously used native E. coli asparaginase product and since two different randomized studies, consisting of PEG-asparaginase-intensified schedules, are the most relevant treatment questions of the AIEOP-BFM ALL 2009 study, a tight therapeutic drug monitoring study of PEG-asparaginase treatment has been implemented to better understand the pharmacological phenomena underlying asparaginase treatment in this therapeutic context.

The main findings of the above-mentioned therapeutic drug monitoring specifically related to CSF asparagine levels and asparaginase serum activity, analyzed in parallel after the administration of PEG-asparaginase in the induction phase of the AIEOP-BFM ALL 2009 study, are the focus of the present report.

Methods

Patients’ eligibility and treatment schedule

Children ≥1 year and <18 years old diagnosed with ALL and eligible for the AIEOP-BFM ALL 2009 protocol were investigated in this study. PEG-asparaginase (Oncaspar, Shire) was given during the induction phase (namely protocol IA) to children diagnosed and treated in the participating centers. The drug was given intravenously as a 2 h infusion at the dosage of 2,500 IU/m with a maximum dose of 3,750 IU/m on days 12 and 26. Details of the treatment are available in the European Clinical Trials Database at https://www.clinicaltrialsregister.eu/ctr-search/trial/2007-004270-43/IT. CSF asparagine levels were evaluated when lumbar punctures relevant for this part of the PEG-asparaginase study were scheduled in protocols IA and the subsequent consolidation phase protocol IB, i.e., on protocol days +33 and +45, respectively, which correspond to days 7 and 19 after the second PEG-asparaginase dose of protocol IA. Serum asparaginase activity levels were measured at the same two time points. Mainly because of the long half-life of PEG-asparaginase and the slow decay of the related activity levels, and in order to have a larger set of samples to be analyzed, data analyses were focused on these two time points only but with the following adjustments: (i) CSF samples were considered analyzable when collected at a distance of 7±3 days and of 19±3 days after the second PEG-asparaginase dose (day +26) of protocol IA; (ii) the serum samples had to be collected the same day (±1) as the CSF samples. In the text, tables and figures of this report the CSF asparagine values obtained at day +33 ±3 and day +45 ±3 are simply referred to as day +33 and day +45.

Sample collection

Serum and CSF sample collection started on June 1, 2010; CSF collection ended on December 31, 2012. Samples were collected from patients treated according to the AIEOP-BFM ALL 2009 protocol in Italy (AIEOP), Germany (BFM-G), Austria (BFM-A), and the Czech Republic (CPH). CSF samples were immediately frozen at −80°C, shipped on dried ice and stocked at −80°C until amino acid analysis. Blood samples from a peripheral vein or central venous catheter were collected according to the treatment schedule. Serum was separated in 2 mL tubes and immediately frozen at −20°C until shipment. CSF asparagine levels and asparaginase serum activity were determined in the Laboratory of Cancer Pharmacology at the Department of Oncology of the “Mario Negri” Pharmacology Research Institute IRCCS (Milan, Italy) for the AIEOP samples, in the Clinical Pharmacology Laboratory of the Department of Pediatric Hematology and Oncology at the University Hospital of Muenster (Germany) for the BFM-G and CPH samples and in the Department of Pediatrics and Adolescent Medicine of the Medical University of Vienna (Austria) for the BFM-A CSF samples.

Determination of serum pegylated-asparaginase activity

PEG-asparaginase activity was evaluated with the commercially available enzymatic medac asparaginase activity test (MAAT) (medac GmbH, Hamburg, Germany) or with the L-aspartic β-hydroxamate (AHA) test.17

The medac asparaginase activity test

Briefly, the MAAT is an IVD-CE-certified test which is commercially available. It is a homogeneous microplate assay that analyses the catalytically active asparaginase in serum by detecting the amount of hydrolyzed substrate analogue of asparagine, quantified by photometric reading at 700 nm. The assay uses calibrators containing a native enzyme preparation from E. coli (ASP medac) and has a lower limit of quantification (LLOQ) of 30 U/L. All the values below the LLOQ were considered 0 U/L for the statistical analysis. The MAAT was used for the determination of asparaginase activity in the serum samples of AIEOP patients.

The L-aspartic β-hydroxamate test

AHA is the substrate for the quantification of native E. coli, pegylated E. coli, and Erwinia chrysanthemii asparaginase in human serum. Asparaginase hydrolyzes AHA to L-aspartic acid and hydroxylamine, which is determined at 710 nm after condensation with 8-hydroxyquinoline and oxidation to indooxine. The LLOQ is 5 U/L.17 All the values below the LLOQ were considered 0 U/L for the statistical analysis. The AHA test was used for the determination of asparaginase activity in serum of CPH and BFM-G samples. Since the AHA test calibrates against known amounts of PEG-asparaginase in contrast to the MAAT, which uses native E. coli asparaginase as the calibrator, it considers the different substrate turnover rates of PEG-asparaginase compared to native E. coli asparaginase under the assay conditions. Thus, the PEG-asparaginase activity determined by the MAAT is a mean of 1.42 higher than that determined by the AHA test, as recently demonstrated.18

Determination of cerebrospinal fluid asparagine levels

CSF asparagine levels were measured using a high performance liquid chromatographic technique after derivatization with o-phthaldialdehyde as described by Turnell and Cooper19 and already used in previous pharmacological studies performed by the AIEOP-BFM group.2015 The LLOQ was 0.2 μmol/L and all the analyzed data with results below this limit were considered 0 μmol/L for the statistical analysis. Since bloody CSF punctures might have altered the quantification of asparagine, either though the release of asparagine present in the erythrocytes or through possible contamination by asparaginase, CSF samples contaminated with blood were excluded from the analysis.

Informed consent

All patients and their parents or legal guardians signed appropriate informed consent for the biological study procedure encompassed in the AIEOP-BFM ALL 2009 study for the asparaginase therapeutic drug monitoring. Assent was given by patients according to ethical standards and national guidelines. Protocol studies were approved by each national and local review board, in accordance with the Declaration of Helsinki and national laws.

Statistical analysis

Descriptive analyses include the distribution of patients’ characteristics and dot plots on CSF asparagine concentration and PEG-asparaginase serum activity. Box plots and scatter plots were used to describe continuous values, with the Wilcoxon test to compare medians. Data are presented separately on the original scale according to the type of enzymatic test used, which was MAAT for AIEOP samples and AHA for all other samples, collectively identified as BFM samples.

Results

Between June 2010 and December 2012 1,764 patients were unselectively enrolled in Italian, German, Czech, and Austrian centers adopting the AIEOP-BFM ALL 2009 study protocol. Overall, 736 patients were included in the present study, 245 of whom belonged to the AIEOP cohort and 491 to the BFM cohort. Their main biological and clinical characteristics are presented in Table 1. The distribution of these characteristics is superimposable to that of the entire cohort of 1,764 patients enrolled in the study in the same period (data not shown).

Table 1.Main biological and clinical characteristics at the onset of acute lymphoblastic leukemia in 736 patients enrolled in the AIEOP-BFM ALL 2009 protocol with at least one cerebrospinal fluid sample. Data are reported separately for the cohorts of patients belonging to the Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and Berlin-Frankfurt-Münster (BFM) groups.

The total number of CSF samples collected in the two groups was 903. Overall, 903 CSF samples were collected on days 33 and/or 45, of which 314 in the AIEOP cohort and 589 in the BFM cohort.

Asparagine levels in cerebrospinal fluid

Of the 903 CSF samples analyzed for asparagine levels, 686 (AIEOP n=230 and BFM n=456) were collected on protocol day +33 and 217 (AIEOP n=84 and BFM n=133) on protocol day +45. The distribution of different CSF asparagine levels detected at the CSF punctures (on days +33 and +45) is presented in Table 2 and Figure 1 (A and B for the AIEOP and BFM cohorts, respectively). Given that the physiological concentration of asparagine in the CSF of children and adolescents ranges between 4 and 10 μmol/L, the CSF asparagine levels found in this study were overall quite consistently reduced at both time points, as depicted in Figure 1. Independently of the levels of asparaginase activity, CSF asparagine levels were significantly reduced during the investigated study phase but only 28% of analyzed samples showed complete asparagine depletion (i.e. below the LLOQ) while relevant levels (≥1 μmol/L) were still detectable in around 23% of them. In particular, asparagine levels ≥1 μmol/L were detected at days +33 and +45 in 16.9% and 34.6% (AIEOP, Table 2A) and in 18.9% and 41.4% (BFM, Table 2B) of analyzed CSF samples, respectively. Median levels were significantly higher at day +45 than at day +33 (AIEOP, P<0.001; BFM, P<0.001).

Table 2.Distribution of asparagine levels in cerebrospinal fluid, at each sampling point (days +33 and +45) in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Figure 1.Asparagine levels in the cerebrospinal fluid during the induction phase. Box plots of asparagine levels (μmol/L) of cerebrospinal (CSF) punctures scheduled on days +33 and +45 in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Asparaginase activity in serum and correlation with cerebrospinal fluid asparagine levels

Overall there were 753 serum samples (AIEOP n=271 and BFM n=482) corresponding to the available CSF samples of which 574 (AIEOP n=198 and BFM n=376) were collected on day +33 and 179 (AIEOP n=73 and BFM n=106) on day +45. The mean PEG-asparaginase activity levels measured in these serum samples were 1,839 (±685) IU/L and 314 (±266) IU/L at days +33 and +45 in AIEOP samples (MAAT) and 1,226 (±470) IU/L and 222 (±141) IU/L in BFM samples (AHA test), respectively. PEG-asparaginase activity <100 IU/L was found in 1.9% of serum samples (2.5% in AIEOP and 1.6% in BFM) taken at day +33 and in 19.6% of serum samples (17.8% in AIEOP and 20.8% in BFM) taken at day +45 (Table 5A,B)

As shown in Table 3A (for the AIEOP cohort) and 3B (for the BFM cohort), at serum asparaginase activity levels <100 IU/L, 100% and 89.3% of the respective patients had CSF asparagine levels >0.2 μmol/L, while this rate decreased to approximately 70% at asparaginase activity ≥100 IU/L. Figures 2 and 3 (subdivided in A and B for the AIEOP and BFM cohorts, respectively) show the CSF asparagine levels at days +33 and +45 in relationship to the asparaginase activity detected at the same time points. At serum asparaginase activity levels lower than 100 IU/L the median CSF asparagine concentration was higher than that in the cohorts with serum activity above 100 IU/L and below 500 IU/L (P<0.003 for AIEOP and P<0.002 for BFM) and that with an overall activity level above 100 IU/L (P<0.001). When asparaginase activity and CSF asparagine levels were determined using progressively higher activity level intervals, even at high asparaginase serum levels of ≥1,500 IU/L, CSF asparagine levels below the LLOQ were found in roughly one-third of the samples (Table 3A and B), indicating that the asparagine level in the CSF was above the LLOQ even at higher levels of asparaginase activity in serum.

Table 3.Asparagine levels in cerebrospinal fluid punctures scheduled on days +33 and +45 sorted according to respective serum asparaginase activity levels in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Figure 2.Effect of pegylated-asparaginase activity on asparagine level in the cerebrospinal fluid. Distribution of asparagine levels (μmol/L) detected in cerebrospinal (CSF) samples collected during puncture on days +33 (blue dots) and +45 (red dots) versus pegylated asparaginase (PEG-ASP) activity levels (IU/L) detected in serum at the same sampling day (±1) in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Figure 3.Cerebrospinal fluid asparagine concentration at different levels of pegylated-asparaginase activity. Box plots of asparagine cerebrospinal fluid (CSF) concentrations (μmol/L) versus categorized pegylated-asparaginase (PEG-ASP) activity levels (IU/L) in serum collected at the same sampling points (±1 day) in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Of note, the data on the relationship between serum asparaginase activity and CSF asparagine levels obtained in the two cohorts of patients were consistent within subgroups defined by clinical and biological characteristics, such as sex, age, white blood cell count at diagnosis and immunophenotype (Table 4).

Table 4.Asparagine levels in cerebrospinal fluid sorted by asparaginase activity levels in serum, at scheduled cerebrospinal fluid punctures (days +33 and +45) in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Table 5 shows asparagine levels in CSF according to whether the asparaginase activity in the serum was less than 100 IU/L or above this level at days +33 and +45 in (A) AIEOP and (B) BFM cohorts. The asparagine levels in CSF samples were significantly higher when serum asparaginase activity was below 100 IU/L than when it was higher than 100 IU/L in both cohorts (AIEOP and BFM).

Table 5.Asparagine levels in cerebrospinal fluid by levels of asparaginase activity in serum, at the cerebrospinal fluid sampling points (days +33 and +45) in the (A) Associazione Italiana di Ematologia e Oncologia Pediatrica (AIEOP) and (B) Berlin-Frankfurt-Münster (BFM) cohorts.

Discussion

Survival rates obtained with chemotherapy schedules applied over the last three decades in childhood ALL have increased progressively and currently approach 90%.3

Asparaginase has been shown to play a key role in obtaining such excellent results and for this reason the drug has been invariably included, since its introduction in clinical practice, in the polychemotherapy schedules designed for childhood ALL. The enzyme exerts its antileukemic activity by depleting the systemic pools of asparagine, an amino acid essential for the rapid proliferation of malignant lymphoblasts.2321

It is well known that the activity of any asparaginase product may be pharmacologically monitored by measuring serum asparaginase activity levels, which reflect the enzyme’s ability to deplete circulating asparagine pools and are considered a surrogate marker of its clinical efficacy.1 There is currently a wide agreement that activity levels of at least 0.1 IU/mL (i.e. 100 IU/L) should be achieved and maintained during the whole planned asparaginase treatment to ensure maximal asparagine depletion in serum (<0.2 μmol/L) and maximal therapeutic efficacy.219 Whether a similarly profound and prolonged asparagine depletion in the CSF is needed to prevent CNS relapses is not known; however, there are reports associating the two phenomena.4

The physiological concentration of asparagine in human CSF varies depending on the age of the patient. In children and adolescents its concentration ranges between 4 and 10 μmol/L.24 Although these values are lower than those found in serum (about 40-80 μmol/L), it has been reported that these levels ensure the growth of leukemic blasts.25 For this reason, in principle, it is reasonable to study asparagine depletion in CSF to evaluate its clinical relevance better and prospectively.

The main purpose of the study reported here was to evaluate the level of asparagine depletion in the CSF and therefore the pharmacodynamic effect exerted by PEG-asparaginase on the CNS of children with ALL. The interest in this aspect derives from various studies showing that different degrees of asparagine depletion in the CSF may depend not only on the asparaginase product used94 but, apparently, also on the levels of asparaginase activity achieved in serum.2826

In this study the administration of PEG-asparaginase in the induction phase of the ALL treatment adopted was associated with a significant, even if widely variable, reduction of CSF asparagine below the physiological levels. However, complete asparagine depletion was observed overall in only about 28% of the analyzed CSF samples. Considerable CSF asparagine levels, greater than 1 μmol/L, and thus higher than the LLOQ of the assay used, which is considered the threshold of complete asparagine depletion, were detected overall in 23% of the analyzed CSF samples, with this latter figure becoming 17-19% and 35-41% for samples taken 7 and 19 days, respectively, after PEG-asparaginase administration (Table 2A,B).

The findings of the large therapeutic drug monitoring program regarding asparaginase activity levels in serum conducted in the frame of the AIEOP-BFM ALL 2009 study and here reported regard exclusively the subset of patients studied to evaluate asparagine depletion in the CSF. These data show that after a dose of 2,500 IU/m, PEG-asparaginase activity levels much higher than 100 IU/L are achieved in induction in the vast majority of patients and are maintained both 7 and 14 days following a standard administration schedule including PEG-asparaginase, thus fully confirming the prolonged half-life of this product (Table 5A,B).

In the serum samples collected along with CSF samples, PEG-asparaginase activity less than 100 IU/L was only detected in around 5-6% of samples, when the samples were taken ≤19 days after administration of PEG-asparaginase (Tables 3A,B and 5A,B). We can, therefore, assume that serum asparagine levels of patients enrolled in this pharmacological study were continuously depleted for at least 14 days after each PEG-asparaginase dose in the majority of the patients.

In our study when CSF asparagine levels were evaluated in relationship to serum asparaginase activity levels, a considerable number of samples was found not to have levels below the LLOQ. In patients with serum asparaginase activity levels below 100 IU/L (which is considered insufficient to consistently obtain complete asparagine depletion in serum) only 6.5% of the corresponding CSF samples had levels below the LLOQ. When the level of asparaginase activity was 100 IU/L or higher, 70% of the samples had asparagine levels higher than 0.2 μmol/L (i.e. higher than the LLOQ). Furthermore, at serum asparaginase activity levels of 100 IU/L or higher – including samples with activity levels greater than 1500 IU/L - only about one third of the corresponding CSF samples had asparagine levels below the LLOQ.

Some studies have been conducted in the past on aspects related to CSF asparagine depletion along with administration of different asparaginase products. Dibenedetto et al. evaluated CSF asparagine levels 3 days after the administration of the fourth dose of ERW- sparaginase (given at a dosage of 10,000 IU/m intramuscularly every 72 h) and found them to be below the LLOQ (≤0.2 μmol/L) in 75% of treated children. Despite the small number of cases analyzed in that experience and based on the fact that asparaginase is believed not to be able to cross the barrier between blood and CSF, it was concluded that this phenomenon was the reflection of the asparagine depletion observed in serum.7 On the other hand, Ahlke et al. showed that 2,500 IU/m un-pegylated E. coli asparaginase led to complete depletion of CSF asparagine 2 or 3 days after application. Median trough plasma activity levels in this dose-group were 106 IU/L (26-349 IU/L).29 Among the findings of our study, we observed that even at asparaginase activity levels greater than 1500 IU/L CSF asparagine levels below the LLOQ were found in roughly 30 to 40% of the samples (Table 3).

In the following years, two additional studies investigated this phenomenon in patients treated with asparaginase. The first, conducted in 1996 by Gentili et al.,5 evaluated 44 patients with newly diagnosed ALL treated in the induction phase of a BFM-oriented protocol with 10,000 IU/m of ERW-asparaginase every 3 days. The analysis of CSF and serum asparagine levels, measured on average 3 days after each dose, revealed CSF asparagine levels similar to those reported in the previously reported study by Dibenedetto et al.7 The second study, performed by Rizzari et al.,6 compared the ability of ERW-asparaginase and native E. coli asparaginase to deplete asparagine in the CSF. In all the 62 patients treated in the induction phase with either intravenous or intramuscular ERW-asparaginase or native E. coli asparaginase (10,000 IU/m every 3 days), asparagine levels in both the serum and CSF remained below the LLOQ (≤0.2 μmol/L) even if asparaginase activity levels were higher in the group treated with E. coli asparaginase than in that treated with ERW-asparaginase. Similar results were found in a study by Woo et al.8

A different trend has been found in studies performed so far in patients treated with PEG-asparaginase. Vieira Pinheiro et al.30 studied patients treated with PEG-asparaginase within the German Cooperative Acute Lymphoblastic Leukemia (COALL) study and Rizzari et al.15 patients treated with the same product within the AIEOP ALL 2000 study. Overall, both studies showed that CSF asparagine levels in patients treated with PEG-asparaginase were undetectable (i.e., below the detection limit) only in a fraction of patients, no matter if serum asparaginase activity levels were much higher than 100 IU/L. Additional studies reported by the Nordic Society of Pediatric Hematology and Oncology and even more recently by the Dutch Childhood Leukemia Study Group (DCLSG) confirmed these observations.32312714

Based on the most updated scientific evidence it is not possible to provide a clear and incontrovertible explanation on how asparaginase products may achieve the observed asparagine depletion in the CSF. It has been hypothesized that the asparagine depletion observed in the CSF could result from a continuous balance between the serum and CSF asparagine pools.1110 Another possible explanation can be inferred from the specific physicochemical properties of the native asparaginase products compared to the PEG-asparaginase product. It is conceivable that native asparaginase formulations, given their lower molecular weight and steric size, might have some capacity to penetrate, even in very low amounts, into the CSF thus providing local asparaginase activity. Nevertheless, it has been postulated that this activity never exceeds 0.2% of that present in serum.11 Conversely, this may not be possible for PEG-asparaginase, mainly because of its tertiary structure.333216 However, so far there is no clear proof that any asparaginase product determines any degree of CSF asparagine depletion in humans by directly penetrating the CSF. To contribute to this issue a preclinical study was recently conducted to evaluate whether the three commercially available asparaginase formulations have different abilities to enter the CSF and reduce local asparagine levels. Even with the limitations of the model used in that preclinical experience, the enzymatic activity measured in CSF demonstrated that asparaginase products, in particular both the native forms derived from Erwinia chrysanthemi and E. coli, may transiently penetrate the CNS when administered at high doses, whereas the PEG-asparaginase product does not, most probably because of the differences in molecular weight.353416

To conclude, the findings of the therapeutic drug monitoring performed in our study and reported here indicate that: (i) the administration of PEG-asparaginase was able to cause a broad reduction of physiological CSF asparagine levels (normally 4-10 μmol/L) but complete asparagine depletion was observed overall in only about 28% of the analyzed CSF samples; (ii) CSF asparagine levels greater than 1 μmol/L (thus higher than the LLOQ of the assay adopted) were detectable in 23% of the analyzed samples; (iii) at serum asparaginase activity levels less than 100 IU/L only 6.5% of the CSF samples had asparagine levels below the LLOQ; and (iv) at serum asparaginase activity levels of 100 IU/L and higher, up to 1,500 IU/L and beyond, CSF asparagine levels were lower than the LLOQ in only about 33-37% of the samples. Thus, a further increase of the PEG-asparaginase dose would not help to obtain complete CSF asparagine depletion.

The consistent results found in the two independent data sets presented here strengthen the observations inferred from this study.

Acknowledgments

The authors thank the patients and families who participated in this trial, the physicians and nurses of all hospitals for their contribution in performing this study, and the members of the AIEOP-BFM ALL 2009 Asparaginase Working Party for productive discussions during the development and progress of the study. They also thank the partners in the reference laboratories and all the technicians for their expert work in cytology, genetics, and MRD diagnostics; and the data managers for their careful study conduction.

Footnotes

  • ^ CR and CL-K share first authorship.
  • * MZ and JB share last authorship.
  • Check the online version for the most updated information on this article, online supplements, and information on authorship & disclosures: www.haematologica.org/content/104/9/1812
  • FundingThis study was supported by Comitato M. L. Verga and Fondazione Tettamanti (Monza) and by Stiftung Deutsche Krebshilfe (Bonn).The TDM program performed in the international AIEOP-BFM ALL 2009 study has been supported by an unrestricted grant from the Shire company (and previously from medac GmBH, Sigma-Tau, Baxalta, which marketed the drug during the period of the present study).
  • Received September 14, 2018.
  • Accepted January 31, 2019.

References

  1. Labrou NE, Papageorgiou AC, Avramis VI. Structure-function relationships and clinical applications of L-asparaginases. Curr Med Chem. 2010; 17(20):2183-2195. PubMedhttps://doi.org/10.2174/092986710791299920Google Scholar
  2. Pieters R, Hunger SP, Boos J. L-asparaginase treatment in acute lymphoblastic leukemia: a focus on Erwinia asparaginase. Cancer. 2011; 117(2):238-249. PubMedhttps://doi.org/10.1002/cncr.25489Google Scholar
  3. Pui C-H, Campana D, Pei D. Treating childhood acute lymphoblastic leukemia without cranial irradiation. N Engl J Med. 2009; 360(26):2730-2741. PubMedhttps://doi.org/10.1056/NEJMoa0900386Google Scholar
  4. Avramis VI, Sencer S, Periclou AP. A randomized comparison of native Escherichia coli asparaginase and polyethylene glycol conjugated asparaginase for treatment of children with newly diagnosed standard-risk acute lymphoblastic leukemia: a Children’s Cancer Group study. Blood. 2002; 99(6):1986-1994. PubMedhttps://doi.org/10.1182/blood.V99.6.1986Google Scholar
  5. Gentili D, Conter V, Rizzari C. L-Asparagine depletion in plasma and cerebrospinal fluid of children with acute lymphoblastic leukemia during subsequent exposures to Erwinia L-asparaginase. Ann Oncol. 1996; 7(7):725-730. PubMedhttps://doi.org/10.1093/oxfordjournals.annonc.a010722Google Scholar
  6. Rizzari C, Zucchetti M, Conter V. L-asparagine depletion and L-asparaginase activity in children with acute lymphoblastic leukemia receiving i.m. or i.v. Erwinia c. or E. coli L-asparaginase as first exposure. Ann Oncol. 2000; 11(2):189-193. PubMedhttps://doi.org/10.1023/A:1008368916800Google Scholar
  7. Dibenedetto SP, Di Cataldo A, Ragusa R, Meli C, Lo Nigro L. Levels of L-asparagine in CSF after intramuscular administration of asparaginase from Erwinia in children with acute lymphoblastic leukemia. J Clin Oncol. 1995; 13(2):339-344. PubMedGoogle Scholar
  8. Woo MH, Hak LJ, Storm MC. Cerebrospinal fluid asparagine concentrations after Escherichia coli asparaginase in children with acute lymphoblastic leukemia. J Clin Oncol. 1999; 17(5):1568-1568. PubMedGoogle Scholar
  9. Pinheiro JPV, Boos J. The best way to use asparaginase in childhood acute lymphatic leukaemia–still to be defined?. Br J Haematol. 2004; 125(2):117-127. PubMedhttps://doi.org/10.1111/j.1365-2141.2004.04863.xGoogle Scholar
  10. Schwartz MK, Lash ED, Oettgen HF, Tomato FA. L-asparaginase activity in plasma and other biological fluids. Cancer. 1970; 25(2):244-252. PubMedGoogle Scholar
  11. Riccardi R, Holcenberg JS, Glaubiger DL, Wood JH, Poplack DG. L-asparaginase pharmacokinetics and asparagine levels in cerebrospinal fluid of rhesus monkeys and humans. Cancer Res. 1981; 41(11 Pt 1):4554-4558. PubMedGoogle Scholar
  12. Müller HJ, Boos J. Use of L-asparaginase in childhood ALL. Crit Rev Oncol Hematol. 1998; 28(2):97-113. PubMedhttps://doi.org/10.1016/S1040-8428(98)00015-8Google Scholar
  13. Avramis VI, Panosyan EH. Pharmacokinetic/pharmacodynamic relationships of asparaginase formulations The past, the present and recommendations for the future. Clin Pharmacokinet. 2005; 44(4):367-393. PubMedhttps://doi.org/10.2165/00003088-200544040-00003Google Scholar
  14. Appel IM, Pinheiro JPV, den Boer ML. Lack of asparagine depletion in the cerebrospinal fluid after one intravenous dose of PEG-asparaginase: a window study at initial diagnosis of childhood ALL. Leukemia. 2003; 17(11):2254-2256. PubMedhttps://doi.org/10.1038/sj.leu.2403143Google Scholar
  15. Rizzari C, Citterio M, Zucchetti M. A pharmacological study on pegylated asparaginase used in front-line treatment of children with acute lymphoblastic leukemia. Haematologica. 2006; 91(1):24-31. PubMedGoogle Scholar
  16. Ballerini A, Moro F, Nerini IF. Pharmacodynamic effects in the cerebrospinal fluid of rats after intravenous administration of different asparaginase formulations. Cancer Chemother Pharmacol. 2017; 79(6):1267-1271. Google Scholar
  17. Lanvers C, Vieira Pinheiro JP, Hempel G, Wuerthwein G, Boos J. Analytical validation of a microplate reader-based method for the therapeutic drug monitoring of L-asparaginase in human serum. Anal Biochem. 2002; 309(1):117-126. PubMedhttps://doi.org/10.1016/S0003-2697(02)00232-4Google Scholar
  18. Lanvers-Kaminsky C, Rüffer A, Würthwein G. Therapeutic drug monitoring of asparaginase activity-method comparison of MAAT and AHA test used in the international AIEOP-BFM ALL 2009 trial. Ther Drug Monit. 2018; 40(1):93-102. Google Scholar
  19. Turnell DC, Cooper JD. Rapid assay for amino acids in serum or urine by pre-column derivatization and reversed-phase liquid chromatography. Clin Chem. 1982; 28(3):527-531. PubMedGoogle Scholar
  20. Boos J, Werber G, Ahlke E. Monitoring of asparaginase activity and asparagine levels in children on different asparaginase preparations. Eur J Cancer. 1996; 32A(9):1544-1550. https://doi.org/10.1016/0959-8049(96)00131-1Google Scholar
  21. Moricke A, Zimmermann M, Valsecchi MG. Dexamethasone vs prednisone in induction treatment of pediatric ALL: results of the randomized trial AIEOP-BFM ALL 2000. Blood. 2016; 127(17):2101-2112. PubMedhttps://doi.org/10.1182/blood-2015-09-670729Google Scholar
  22. Asselin B, Rizzari C. Asparaginase pharmacokinetics and implications of therapeutic drug monitoring. Leuk Lymphoma. 2015; 56(8):2273-2280. Google Scholar
  23. van den Berg H. Asparaginase revisited. Leuk Lymphoma. 2011; 52(2):168-178. PubMedhttps://doi.org/10.3109/10428194.2010.537796Google Scholar
  24. Zeidan A, Wang ES, Wetzler M. Pegasparaginase: where do we stand?. Expert Opin Biol Ther. 2009; 9(1):111-119. PubMedhttps://doi.org/10.1517/14712590802586058Google Scholar
  25. Gerrits GP, Trijbels FJ, Monnens LA. Reference values for amino acids in cerebrospinal fluid of children determined using ion-exchange chromatography with fluorimetric detection. Clin Chim Acta. 1989; 182(3):271-280. PubMedhttps://doi.org/10.1016/0009-8981(89)90104-6Google Scholar
  26. Asselin BL, Lorenson MY, Whitin JC. Measurement of serum L-asparagine in the presence of L-asparaginase requires the presence of an L-asparaginase inhibitor. Cancer Res. 1991; 51(24):6568-6573. PubMedGoogle Scholar
  27. Henriksen LT, Nersting J, Raja RA. Cerebrospinal fluid asparagine depletion during pegylated asparaginase therapy in children with acute lymphoblastic leukaemia. Br J Haematol. 2014; 166(2):213-220. Google Scholar
  28. Hawkins DS. Asparaginase pharmacokinetics after intensive polyethylene glycol-conjugated L-asparaginase therapy for children with relapsed acute lymphoblastic leukemia. Clin Cancer Res. 2004; 10(16):5335-5341. PubMedhttps://doi.org/10.1158/1078-0432.CCR-04-0222Google Scholar
  29. Ahlke E, Nowak-Göttl U, Schulze-Westhoff P. Dose reduction of asparaginase under pharmacokinetic and pharmacodynamic control during induction therapy in children with acute lymphoblastic leukaemia. Br J Haematol. 1997; 96(4):675-681. PubMedhttps://doi.org/10.1046/j.1365-2141.1997.d01-2089.xGoogle Scholar
  30. Vieira Pinheiro JP, Wenner K, Escherich G. Serum asparaginase activities and asparagine concentrations in the cerebrospinal fluid after a single infusion of 2,500 IU/m(2) PEG asparaginase in children with ALL treated according to protocol COALL-06-97. Pediatr Blood Cancer. 2006; 46(1):18-25. PubMedhttps://doi.org/10.1002/pbc.20406Google Scholar
  31. Tong WH, Pieters R, de Groot-Kruseman HA. The toxicity of very prolonged courses of PEGasparaginase or Erwinia asparaginase in relation to asparaginase activity, with a special focus on dyslipidemia. Haematologica. 2014; 99(11):1716-1721. PubMedhttps://doi.org/10.3324/haematol.2014.109413Google Scholar
  32. van der Sluis IM, de Groot-Kruseman H, Te Loo M. Efficacy and safety of recombinant E. coli asparaginase in children with previously untreated acute lymphoblastic leukemia: a randomized multi-center study of the Dutch Childhood Oncology Group. Pediatr Blood Cancer. 2018; 65(8):e27083. Google Scholar
  33. Pasut G, Veronese FM. State of the art in PEGylation: the great versatility achieved after forty years of research. J Control Release. 2012; 161(2):461-472. PubMedhttps://doi.org/10.1016/j.jconrel.2011.10.037Google Scholar
  34. Serlin Y, Shelef I, Knyazer B, Friedman A. Anatomy and physiology of the blood– brain barrier. Semin Cell Dev Biol. 2015; 38:2-6. https://doi.org/10.1016/j.semcdb.2015.01.002Google Scholar
  35. Pardridge WM. Drug transport across the blood-brain barrier. J Cereb Blood Flow Metab. 2012; 32(11):1959-1972. PubMedhttps://doi.org/10.1038/jcbfm.2012.126Google Scholar

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Vol. 104 No. 9 (2019): September, 2019 : Articles
 
DOI
https://doi.org/10.3324/haematol.2018.206433
Pubmed
30705097
Pubmed Central
PMC6717578
 
Published
2019-09-01
Published By
Ferrata Storti Foundation, Pavia, Italy
Print ISSN
0390-6078
Online ISSN
1592-8721
 

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