A group of 52 patients ≤18 years were recruited retrospectively from three pediatric oncology centers in Poland: Lodz, Zabrze and Lublin. The patients were diagnosed with BCP-ALL between December 2005 and January 2016 and treated with the Berlin-Frankfurt-Münster backbone protocols with L-asp as a core regimen (ALL IC, 2002 and 2009) (17,18). Matched DNA and RNA samples from the bone marrow aspiration at the point of diagnosis, as well as clinical data, were acquired. BCR-ABL1 fusion, ETV6-RUNX1 fusion, hypodiploidy and hyperdiploidy were assessed routinely by fluorescence in situ hybridization and karyotyping performed in a certified laboratory (Genetic Laboratory at Collegium Medicum; Bydgoszcz, Poland) at the time of diagnosis. Each patient and/or their parents provided signed informed consent in writing prior to inclusion in the study.

For all collected bone marrow samples, MLPA analysis with P327-B1 iAMP21-ERG probe mix was performed according to the manufacturer's protocol (MRC-Holland BV). Additionally, MLPA P329 CRLF2-CSF2RA-IL3RA and P335 ALL-IKZF1 (MRC-Holland BV) probe mixes for cytokine receptor-like factor 1, IKZF1, IKZF2, IKZF3, cyclin-dependent kinase inhibitor (CDKN) 2A/2B, retinoblastoma 1 (RB1), PAX5 and ETV6 amplification or deletion status detection were used. Absolute fluorescence was normalized by comparing peak patterns of DNA in the sample of interest with a DNA isolated from blood samples from age- and gender-matched healthy individuals who provided written consent to participate in the study. The relative probe ratio of the tested samples was compared with the average relative probe ratio in the reference samples to calculate the dosage quotient. Data analysis and interpretation were conducted using GeneMarker v2.7.4 software (Softgenetics, LLC) according to the manufacturer's protocol.

To obtain cDNA for quantitative PCR, all available RNA samples that were extracted using the TRIzol reagent (Thermo Fisher Scientific, Inc.) were reverse transcribed using a High-Capacity cDNA Reverse Transcription kit (Thermo Fisher Scientific, Inc.). The thermal conditions were 30 min at 50°C, 15 min at 95°C, followed by storage at 4°C. TaqMan Gene Expression assays (Applied Biosystems; Thermo Fisher Scientific, Inc.) for ASNS (cat. no. Hs04186194_m1), LGMN (cat. no. Hs00271599_m1) and CTSB (cat. no. Hs00947433_m1) were used; GAPDH (cat. no. Hs02786624_g1) was selected as a control. The thermocycling conditions were as follows: 50°C for 2 min and 95°C for 10 min, followed by 40 cycles of 95°C for 15 sec and 60°C for 1 min. All samples were tested in duplicate and the 2^−ΔΔCq value was calculated (19) with GAPDH used for normalization. The relative mRNA expression was used for further comparisons.

The search for PAX5 binding sites throughout the human and mouse genome matrix was conducted using the HOCOMOCO v11, TRANSFAC database version 2018.3 (GeneXplain, GmbH). This is an online engine for searches through multiple module databases and was used as previously described (20).

Statistica 12.0 software (TIBCO Software, Inc.) was used for all analyses. Nominal variables are presented as percentages; differences between the groups were evaluated using the χ² test. Continuous variables are presented as medians with interquartile range (IQR); differences between groups were evaluated using the Kruskal-Wallis test and post-hoc Tukey's HSD test or the Mann-Whitney U test for paired groups were used to establish groups with significant differences. Correlations between continuous variables were calculated with the Spearman's rank-correlation coefficient. Kaplan-Meier curves were used to present relapse-free survival (RFS) time, and hazard ratios (HRs) were calculated using Cox proportional hazards. P<0.05 was considered to indicate a statistically significant difference. For the graphical presentation of result, GraphPad Prism 7.05 software (GraphPad Software, Inc.) was used.

A total of 52 children with BCP-ALL were enrolled in the study with a median age at diagnosis of 6.54 years (IQR, 2.97–12.38 years). The group was predominantly male (60.40%). The median white blood cell (WBC) count at diagnosis was 1.40×10⁴ cells/µl (IQR, 0.41–9.68×10⁴ cells/µl) and the median leukemic cell percentage in bone marrow collected at diagnosis assessed by flow cytometry was 93.10% (IQR, 83.50–96.70%). The mean follow-up time was 4.43 years (range, 0.24–9.6 years).

The patient cohort was divided into groups based on the major genetic abnormalities detected in leukemic cells that have prognostic value within the used treatment protocols: The BCR-ABL1 fusion-positive group (n=5; 9.62% of all patients), hyperdiploid group (n=7; 13.46%), hypodiploid (n=2; 3.85%), ETV6-RUNX1 fusion (n=3; 5.77%) and other BCP-ALL group with no clear primary genetic aberrations (n=35; 67.31%) (Table I). The subgroups differed significantly in age at diagnosis, with the BCR-ABL1 fusion group being the oldest at diagnosis (median, 13.76 years; IQR, 6.76–13.90 years; P=0.04).

The incidence of CNVs frequently observed in childhood ALL varied between the groups. All patients in the ETV6-RUNX1 fusion group carried IKZF1 and ETV6 deletions in the leukemic clone, and 2 out of the 3 patients displayed concomitant CDKN2A/2B deletion. The majority of patients with BCR-ABL1 fusion exhibited IKZF1 and PAX5 deletions (both were present in 3 out of 5 patients) and CDKN2A/2B, CRLF2, ETV6, RB1 and transcriptional regulator ERG (ERG) deletions were detected in 1 out of 7 patients each. In the patients from the hyperdiploid group, IKZF1 (3 out of 7), CRLF2 (2 out of 7), CDKN2A/2B (1 out of 7), PAX5 (1 out of 7) and Janus kinase 2 (JAK2; 1 out of 7) deletions were identified. The other BCP-ALL group was the most heterogenic among all groups; all patients exhibited CNVs in at least one of the tested genes with an incidence of 29 for IKZF1, 2 for IKZF2, 2 for IKZF3, 17 for CDKN2A/2B, 8 for PAX5, 4 for CRLF2, 4 for JAK2, 9 for ETV6, 4 for ERG and 6 for RB1 out of 35 patients in this group (Table SI).

Expression levels of ASNS, LGMN and CTSB were measured in diagnostic bone marrow samples from the 52 patients. The median relative expression value for ASNS was 2.57 (IQR, 2.26–3.26), for LGMN was 1.48 (IQR, 1.21–2.14) and for CTSB was 1.14 (IQR, 0.79–1.77). The median relative mRNA expression of ASNS correlated significantly with LGMN and CTSB (r=0.59 and r=0.62, respectively; P<0.05, data not shown. No correlations were identified between ASNS, LGMN and CTSB expression levels and minimal residual disease (MRD) on day 15 of the treatment protocol or RFS time (data not shown). In addition, no relevant differences in the median relative mRNA expression levels of the evaluated genes between the distinct molecular groups of BCP-ALL were identified (Table SII; Fig. 1A-C).

Analysis of the gene expression profiles based on common CNVs revealed a significantly higher median LGMN relative expression level in patients with PAX5 deletion compared with patients with wild-type PAX5 in all BCP-ALL subgroups (median, 1.93 and 1.34, respectively; P=0.0282; Table SIII). Patients with PAX5 deletion also exhibited a significant correlation of CTSB median expression level with ASNS and LGMN (r=0.73 and r=0.64, respectively; P<0.05, data not shown). By contrast, deletion of IKZF1, IKZF2, IKZF3, CDKN2A/2B, CRLF2, JAK2, ETV6, RB1 or ERG did not exhibit predictive significance for ASNS, LGMN and CTSB median expression levels as a single factor (Table SIII).

Differences in ASNS, LGMN and CTSB expression levels in the other BCP-ALL group were identified when the patients were divided into subgroups based on PAX5 deletion status; 8/35 (24%) patients carried PAX5 deletions, whereas 27/35 (76%) did not. Patients with PAX5 deletions exhibited a higher relative expression level of ASNS compared with the wild-type PAX5 group (3.14 vs. 2.47; P=0.0117; Fig. 2A). Similar results were observed for LGMN expression levels, which were higher in patients with PAX5 deletion compared with patients with wild-type PAX5 (2.24 vs. 1.45; P=0.0029; Fig. 2A). In addition, median CTSB expression levels were higher in patients with PAX5-deletions compared with patients with wild-type PAX5 (2.08 vs. 1.04; P<0.0001; Fig. 2A). No significant associations between the median expression levels of the assessed genes were identified when the other BCP-ALL patient group was divided based on IKZF1 deletion status (82.86% of the group carried deletions; Fig. 2B). However, in cases with concomitant deletions of IKZF1 and PAX5 (14.29% of the group-5 patients carried both deletions), significant differences were observed in ASNS and CTSB expression levels (P=0.0334 and P=0.0358, respectively) but not in LGMN expression levels (P=0.0735) (Table SIV; Fig. 2C).

Of the 12 BCP-ALL patients with PAX5 deletion, four deletions were partial and heterozygous and eight affected the whole gene: Seven were heterozygous and one was homozygous. Additionally, TRANSFAC software (GeneXplain, GmbH) was used to test the PAX5 transcription factor binding sites (TFBS) for a possible association with ASNS, LGMN or CTSB. A search through human and mouse databases revealed that the three genes of interest were not directly regulated by PAX5.

In the analyzed cohort of 52 patients, eight relapsed. Median time to relapse was 2.27 years (IQR, 1.37–3.04 years). All relapses occurred in patients in the other BCP-ALL group. RFS did not differ significantly when patients in the other BCP-ALL group were divided according to PAX5 deletion status; median RFS was 5.14 in cases with PAX5 deletion and 5.10 in PAX5 wild-type cases (P=0.4540; HR, 1.56; 95% CI, 0.24–10.20). Out of the eight relapses, six (75%) occurred in patients with wild-type PAX5, whereas two (25%) occurred in patients with PAX5 deletions (P=0.0002). When the impact of PAX5 deletion on RFS was analyzed in the entire cohort, no significant differences were identified (median RFS for wild-type PAX5, 4.69 vs. 4.26 years in cases with PAX5 deletion; P=0.7084; HR, 1.50; 95% CI, 0.22–10.03).

The cohort was divided based on the expression levels of ASNS, LGMN and CTSB, with the cut-off value set as the median expression for each gene (ASNS, 2.57; LGMN, 1.48; CTSB, 1.14). When median RFS was analyzed in patients with high and low ASNS expression, high ASNS expression was associated with a longer time to relapse (P=0.0315; HR, 0.19; 95% CI, 0.04–0.86; Fig. 3A). The 5-year RFS rate of patients with high ASNS expression was 90.15% (95% CI, 87.90–92.40%), and the 5-year RFS rate of patients with low ASNS expression was 73.34% (95% CI, 69.40–77.30%) (P=0.0164). No significant differences in RFS between patients with high and low LGMN or CTSB expression were observed (P=0.2878; HR, 2.36; 95% CI, 0.54–10.37; and P=0.7714; HR, 1.25; 95% CI, 0.28–5.49, respectively; Fig. 3B and C). Patients with high LGMN expression exhibited a 5-year RFS rate of 88.46% (95% CI, 85.70–91.20%), and those with low LGMN expression exhibited a 5-year RFS rate of 77.54% (95% CI, 74.30–80.80%). Similarly, the 5-year RFS rate was 84.71% (95% CI, 81.70–87.70%) for patients with high expression of CTSB and 80.54% (95% CI, 77.40–83.70%) for those with low CTSB expression.