Small nucleolar RNAs as new biomarkers in chronic lymphocytic leukemia

Background

Small nucleolar RNAs (snoRNAs) and small Cajal body-specific RNAs are non-coding RNAs involved in the maturation of other RNA molecules. Alterations of sno/scaRNA expression may play a role in cancerogenesis. This study elucidates the patterns of sno/scaRNA expression in 211 chronic lymphocytic leukemia (CLL) patients (Binet stage A) also in comparison with those of different normal B-cell subsets.

Methods

The patterns of sno/scaRNA expression in highly purified CD19⁺ B-cells of 211 CLL patients and in 18 normal B-cell samples - 6 from peripheral blood, and 12 from tonsils (4 germinal center, 2 marginal zone, 3 switched memory and 3 naïve B-cells) - were analyzed on the Affymetrix GeneChip® Human Gene 1.0 ST array.

Results

CLLs display a sno/scaRNAs expression profile similar to normal memory, naïve and marginal-zone B-cells, with the exception of a few down-regulated transcripts (SNORA31, -6, -62, and -71C). Our analyses also suggest some heterogeneity in the pattern of sno/scaRNAs expression which is apparently unrelated to the major biological (ZAP-70 and CD38), molecular (IGHV mutation) and cytogenetic markers. Moreover, we found that SNORA70F was significantly down-regulated in poor prognostic subgroups and this phenomenon was associated with the down-regulation of its host gene COBLL1. Finally, we generated an independent model based on SNORA74A and SNORD116-18 expression, which appears to distinguish two different prognostic CLL groups.

Conclusions

These data extend the view of sno/scaRNAs deregulation in cancer and may contribute to discover novel biomarkers associated with the disease and potentially useful to predict the clinical outcome of early stage CLL patients.

Chronic lymphocytic leukemia (CLL) is a clinically heterogeneous disease. Some patients have an indolent course and may survive for years without treatment, while others have an aggressive and rapidly progressive course [1, 2]. Although the current Rai [3] and Binet [4] staging systems identify patients with high-risk disease, they do not prospectively distinguish patients with potentially evolving disease from those destined to remain stable for decades.

A number of cellular and molecular markers help to classify CLL into biologically and clinically distinct subgroups, and to predict the clinical course of the disease at diagnosis [5]. CLL patients with unmutated (UM-CLL) immunoglobulin heavy chain variable (IGHV) region genes (>98% homology to germline sequences), increased expression of the CD38 cell surface antigen, or of the 70-kd zeta-chain T-cell receptor–associated protein kinase (ZAP-70) experience a shorter therapy-free interval, a more aggressive clinical course, and a shorter survival [6–8]. Specific recurrent chromosomal abnormalities, traditionally detected by Fluorescence in situ Hybridization (FISH), such as deletions at 13q14 (del13), 11q23 (del11), 17p13 (del17), and trisomy 12 (12+) may also represent important independent biomarkers for disease progression and survival [9–13].

In recent years, the discovery of non-coding RNAs (ncRNAs) has provided new tools for the understanding of cancer biology [14]. ncRNAs are functional transcripts that do not code for proteins, but indeed play a major role in regulating gene expression at virtually all levels. Among these, small nucleolar RNAs (snoRNAs) are molecules of 60–300 nucleotides in length that function as guide RNAs for the post-transcriptional methylation and/or pseudouridylation of ribosomal RNAs. Unlike snoRNAs, small Cajal body-specific RNAs (scaRNAs) accumulate within the Cajal bodies (i.e. conserved subnuclear organelles that are present in the nucleoplasm) and can guide both post-transcriptional modifications of small nuclear RNAs. sno/scaRNAs can also target other RNAs including mRNAs. However, a subgroup of so-called “orphan” sno/scaRNAs exists whose function remain to be clarified. Notably, in vertebrates most sno/scaRNAs reside in the introns of protein-coding host genes and are processed out of the excised introns [15].

Experimental evidence has recently shown that sno/scaRNAs dysfunction may have a role in the origin of human cancers [16]. Limited data concerning the involvement of sno/scaRNAs in hematological malignancies have been reported only very recently by us and others [17–22], and are lacking in CLL.

In the present study, we investigated the sno/scaRNA expression profiling in a large and representative prospective series of Binet stage A CLL patients. In addition, we evaluated sno/scaRNAs expression in comparison to that observed in various sub-populations of normal B-cells from tonsils and peripheral blood B-lymphocytes. Finally, the sno/scaRNA expression pattern was correlated with clinical data in order to outline their possible role in CLL prognosis.

Patients

Two hundred and eleven newly diagnosed CLL patients were prospectively enrolled from several Italian Institutions in an observational multicenter study (O-CLL1 protocol, clinical trial.gov identifier NCT00917540) from January 2007 to May 2011. The National Cancer Institute (NCI)-sponsored Working Group guidelines were followed for diagnosis and staging [23]. All patients had an absolute lymphocyte count (ALC) greater than 5000×10⁹/L in the peripheral blood. Exclusion criteria were the following: i) a CLL diagnosis exceeding 12 months before registration; ii) a leukemic phase of lymphoproliferative disorders of B origin, CD5^- and/or CD23^- according to flow cytometry analysis; iii) a clinical Binet stage B or C; iv) need of therapy according to NCI guidelines and v) age > 70 years. The median follow-up of this series was 30 months. Diagnosis was confirmed by the biological review committee according to flow cytometry analysis centralized at the National Cancer Institute (IST) Laboratory in Genoa. Written informed consent was obtained from all patients in accordance with the declaration of Helsinki and the study was approved by the local Ethics Review Committee (Comitato Etico Provinciale, Modena, Italy).

Peripheral blood mononuclear cells from CLL patients and normal control, and B-cell sub-populations from tonsils (i.e. naïve B-cells (N), marginal zone (MZ)-like, germinal center (GC) and switched memory (SM) B-cells) were obtained as described in Additional file 1 and Additional file 2.

Biological and molecular analyses were performed in highly enriched CD19⁺ B-cells as previously described [24, 25]. CD38 and ZAP-70 expressions were investigated using a cut-off of 20% and 30% respectively to discriminate positive from negative patients. Del11, del13, del17, and 12+, IGHV mutation status and stereotyped BCR subtypes were determined as previously described [26–28]. Specifically, IGHV sequences from 210 patients were submitted to IMGT V-QUEST analysis software, and were classified as mutated (M-CLL) or UM-CLL using a discriminating mutation cut-off percentage at 2%.

Gene expression profiling (GEP)

Total RNA from purified CD19⁺ B-cells of 211 CLL cases and 18 normal B-cell samples - 6 from peripheral blood, and 12 from tonsils (4 germinal center, 2 marginal zone, 3 switched memory and 3 naïve B-cells) - were analyzed on the GeneChip® Human Gene 1.0 ST array (Affymetrix Inc., Santa Clara, CA). The raw intensity expression values were processed by Robust Multi-array Average (RMA) procedure [29] with the re-annotated Chip Definition Files (CDF) from BrainArray libraries version 15.0.0 [30] available at http://brainarray.mbni.med.umich.edu. This custom CDF reorganized probe sets based on i) more stringent gene/transcript definitions from UniGene database, and ii) alignment analyses performed on each single probe included in the probeset [30]. The updated annotations provided a better precision and accuracy in transcript expression level estimates compared to the original Affymetrix definitions [19, 31].

Supervised analyses were carried out using the Significant Analysis of Microarrays software version 4.00 (SAM; excel front-end publicly available at http://www-stat.stanford.edu/~tibs/SAM/index.html) [32]. The cutoff point for statistical significance (at a q-value 0) was determined by tuning the Δ parameter on the false discovery rate and controlling the q-value of the selected probes. Hierarchical agglomerative clustering of the most significant probesets found was performed adopting Pearson and average as distance and linkage methods, respectively. DNA-Chip Analyzer software (dChip) [33] was used to perform clustering and to graphically represent it. GEP data have been deposited in the NCBI Gene Expression Omnibus database (GEO; http://www.ncbi.nlm.nih.gov/geo/) under accession #GSE46261.

In order to explore the distribution of CLL samples we applied principal component analysis (PCA) on sno/scaRNA microarray expression data. PCA was performed by means of the princomp function in R software, by scaling data and using the associated correlation matrix. Hence we used the 3dplot to visualize samples by the first three principal components.

Statistical analysis

We used the Cox proportional hazards model in the globaltest function of R software (with 100,000 permutation) to test the association (positive or negative) between sno/scaRNA expression levels, assumed as continuous variables and progression free survival (PFS) as clinical outcome. The list of significant associated sno/scaRNA to the PFS was reduced to derive a smaller prognostic sno/scaRNA signature by employing single sno/scaRNA expression profile. Unsupervised K-means clustering was applied to each sno/scaRNA to define a threshold splitting samples with higher expression from those with lower expression (Additional file 3), in order to test their different clinical outcome. The survival distributions of patient groups identified by this approach were tested using the Kaplan-Meier estimator and log-rank test, and P-values were calculated according to the standard normal asymptotic distribution (survdiff function of the survival R package). The Benjamini-Hochberg correction has been applied to consider the false discovery rate that incurred in the multiple testing. Independence between commonly used CLL prognostic factors (IGHV mutational status, ZAP-70, CD38 and unfavorable chromosome aberrations, namely del11, del17 and 12+) and sno/scaRNAs signature was assessed using multivariate Cox proportional-hazards regression procedure by the coxph function in the survival R package. The robustness of the 2-snoRNA model was tested using the linear discriminant analysis for the classification of multivariate observations, with leave-one-out procedure, using ldafunction in MASS R package. Other statistical procedures were applied using standard functions in base R package (Kendall Tau correlations and Wilcoxon rank-sum tests).

Characteristics of CLL patients

Two hundred eleven CLL patients at Binet stage A were included in the study; most of them were Rai 0 stage (74.4%). The median follow-up was 30 months (range 1–65 months). CLL cell samples were characterized for IGHV somatic mutations, ZAP-70 and CD38 expression and the presence of typical chromosomal aberrations (del13, del11, del17, and 12+) detected by FISH analysis. Table 1 summarizes the features of CLL samples.

sno/scaRNA expression profile of CLL cells compared to normal B-cell populations

The expression profiles of sno/scaRNA genes were investigated using Human Gene 1.0 ST arrays. Oligonucleotide probes were mapped according to the genome and transcriptome information from the human genome build release GRCh37/hg19 (see Methods) identifying 215 human snoRNA (76 SNORA and 139 SNORD transcripts) and 17 human scaRNA genes. The expression patterns also were studied in normal B-cells from peripheral blood (pBC) and in different tonsil B-cell sub-populations including germinal center (GC), naïve (N), marginal zone (MZ) and memory (SM) B-cells (Additional file 2 reports the FACS sorting strategy used to purify these cell subpopulations as described in Additional file 1).

At first, we applied PCA on the sno/scaRNA dataset composed by 211 CLL and 18 normal cell samples; the first three PCs contained 51% of variance in our data and we used them to display all the cell type samples in a three-dimensional plot. As shown in Figure 1A, we observed that CLL, N, MZ and SM B-cell samples were clustered together, whereas GC and in particular pBC samples, were well-separated from other groups along PC3 and PC1 components, respectively. Based on this evidence, multiclass analysis was performed comparing CLLs with N, MZ and SM (taken as a single group) and GC B-cells. Despite the heterogeneity of snoRNAs expression in CLL samples, we confirmed that the sno/scaRNA expression profile of CLL was much more similar to N-MZ-SM B-cells rather than to GC (Figure 1A-B). Specifically, we observed the significant down-regulation of SNORA31, -6, -62, and 71C, SNORD37, and -50B in CLL with respect to tonsillar B-cells; however, GC B-cells differed from both CLL and N-MZ-SM B-cells on the basis of a number of down-regulated transcripts, such as SNORD116-1, -116-23, -116-29, -94, and SNORA36A (Figure 1B).

sno/scaRNA expression profile of CLL and normal B-cells. A PCA analysis that includes CLL samples shows that CLLs are closer in a three-dimensional space of similarity to SM, N and MZ tonsillar B-lymphocytes than to other B-cell types, based on the expression of 215 snoRNA and 17 scaRNA genes (A). Heatmap of the differentially expressed sno/scaRNAs in CLL patients, N-SM-MZ B-cells, and GC B-cells. snoRNAs also resulting from two-class supervised analysis comparing CLL and N-SM-MZ B-cells group, are marked with an asterisk (B).

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Notably, SNORA31, -6, -62, and -71C also resulted significantly down-regulated in each of the CLL subgroups stratified according to genetic lesions (del13, del11, del17, 12+ and FISH negative) in a two-class supervised analysis with the N, MZ and SM group (data not shown). Finally, in agreement with PCA, supervised analysis confirmed the strong differences in sno/scaRNA expression between pBC and CLL samples, showing the up-regulation of 102 sno/scaRNAs and the down-regulation of a single transcript (SNORA36C) in CLL patients (Additional file 4).

Global sno/scaRNA expression profiling in CLL patients

To determine whether the natural grouping of global sno/scaRNA expression profiling could be associated with particular CLL subgroups, we performed an unsupervised analysis using conventional hierarchical agglomerative clustering of 71 snoRNAs and 9 scaRNAs, the average change of which varied at least 1.5-fold in the expression levels from the mean values across the dataset (Additional file 5 and Additional file 6). However, CLL samples appeared scattered along the dendrogram irrespective of any known molecular characteristic.

Consequently, we performed supervised analyses (q value = 0) to investigate the occurrence of specific sno/scaRNA expression patterns in CLL groups stratified according to the presence/absence of different prognostic markers; i.e. IGHV gene mutations and ZAP-70 and CD38 expression. Significant differences were detected only in the expression of a limited number of transcripts in the groups stratified as above (Table 2). Specifically, UM-CLLs showed the down-regulation of SNORA70F and SNORA70C, and the up-regulation of SNORA71C. Of note, SNORA70F also was found down-regulated in ZAP-70 positive and in CD38 positive CLL patients, in whom SNORA70C was also down-regulated. Furthermore, snoRNAs expression was investigated in cases stratified according to the presence of chromosomal alterations such as 12+, del11, del13, and del17 by supervised analyses (at q value = 0). SNORA70F was significantly down-regulated in CLL patients with 12+ or del11 (Table 2). Overall, lower expression levels of SNORA70F were associated with the cumulative adverse biological and molecular features (see Additional file 7). Moreover, 12+ patients displayed the significant down-regulation of SCARNA17 and up-regulation of three snoRNAs located on chromosome 12 (SNORA2B, SNORD59A, and -59B) (Table 2). The significant down-regulation of SCARNA9 which is located at 11q21 (Table 2), was also observed in cases with del11. Interestingly, in 8/13 del11 cases, for which genome-wide data were available, we observed that the SCARNA9 locus was included in the deleted region (data not shown). By comparing patients with/without del13 we identified 17 snoRNAs and 2 scaRNAs consistently down-regulated in del13 samples (Table 2). Finally, supervised analysis of CLL samples with del17 did not show any differentially expressed sno/scaRNAs, a finding that could be, however, related to the low number of cases.

Correlation of sno/scaRNAs expression levels with those of their corresponding host genes

The vast majority of human sno/scaRNAs are encoded sense-oriented in introns of so-called host genes, and are produced by exonucleolytic processing of the debranched intron after splicing. This suggests that sno/scaRNAs and their host genes may have a coordinate expression. Among 169 sno/scaRNA-host gene couples present on Human Gene 1.0 ST array, we identified by means of the non parametric Kendall τ correlation test, 75 snoRNAs and 4 scaRNAs whose expression levels were significantly correlated with those of their corresponding host genes (Additional file 8); this list includes 15 sno/scaRNAs resulting from the supervised analyses carried out in our study (Table 3). Specifically, SNORA2B and the SNORD59A, -59B cluster, all of which located at 12q13, were up-regulated in patients with 12+ together with their corresponding host transcripts c12orf41 and ATP5B (mitochondrial ATP synthase). Similarly, the expression of SNORA31, which is located at 13q14, was correlated with that of the host gene TPT1. Notably, the expression of SNORA70F was significantly associated with that of its host gene COBLL1, whereas the expression of the SNORA6 and −62 cluster was significantly correlated with that of its host gene RPSA.

Identification of sno/scaRNA transcriptional profile with clinical relevance in the definition of high-risk CLLs

The sno/scaRNAs transcriptional profiles were examined in relation to CLL clinical course in 191/211 CLL patients for whom clinical follow-up was almost 6 months. In particular, we evaluated whether a specific sno/scaRNA signature was significantly associated with PFS in our prospective series. To this aim, we determined possible associations between PFS and each of the 80 most variable sno/scaRNAs across the CLL dataset (i.e. sno/scaRNAs whose average ratio of the expression was at least 1.5 folds above the mean values). Of these 80 sno/scaRNAs, 5 showed significant association with PFS (P < .05, see Additional file 5), i.e. SNORD116-18, SNORA70F, SNORA74A, SNORD56, and SNORD1A.

As a further validation, the expression levels of SNORD1A, and SNORA74A were evaluated in 50 samples by quantitative real time PCR (qRT-PCR) as previously described [19]: the linear correlation analysis indicated a good correspondence between the two techniques (Pearson’s correlation coefficient of 0.71 and 0.76, respectively; data not shown).

Therefore, we focused on each of the 5 snoRNAs as unique predictive factor. Based on the K-means clustering stratification of CLL cases into two groups according to snoRNAs expression level, we found that each snoRNA resulted capable of providing significant predictive value related to PFS in the univariate log-rank test (P < .05, Table 4). However, in multivariate analysis, only SNORA74A, SNORD116-18 and SNORD56 retained their independence (Additional file 9). Specifically, high expression of SNORA74A and SNORD116-18, and low expression of SNORD56 were associated with shorter PFS. We therefore focused on SNORA74A and SNORD116-18, whose ratio between median high- and low-expression levels exceeded two-fold (Additional file 3), to evaluate whether their combination could improve the robustness of the single-snoRNA model, based on the scheme of three groups defined by (i) high/high, (ii) low/low or (iii) discordant expression levels. Significantly, better PFS was identified in patients with the concomitant low expression of SNORA74A and SNORD116-18, whereas no difference emerged between the two other groups, namely those including patients with high expression of both or one of the two snoRNAs (data not shown). Based on these findings, we could define a low-risk group that included 110 patients (58%) characterized by the low expression of both snoRNAs, and a high-risk group (81 patients) characterized by the high expression of at least one of the two snoRNAs. The high-risk group had a hazard ratio of 2.53 (95% CI: 1.48-4.32) and a median PFS of 39 months (Table 5 and Figure 2), versus a median PFS not reached in low-risk group. The robustness of the 2-snoRNA model was tested by leave-one-out cross validation procedure, which ultimately led to near 90% accuracy.

PFS of patients grouped according to the snoRNAs-based model. Kaplan-Meier curves of the 2 groups defined by the 2-snoRNAs model identifying a low-risk group characterized by the low expression of both snoRNAs and a high risk group characterized by the high expression of at least one of the two snoRNAs. The high risk group has a median PFS of 39 months.

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Multivariate Cox regression analysis was finally performed to test the independence of the 2-snoRNAs risk model from known predictive factors in CLL (IGHV mutational status, ZAP-70 and CD38 expression and unfavorable chromosomal aberration) as covariates. The analysis ascertained the independent prognostic value of the 2-snoRNAs model in our series (p = 0.0007, Table 5).

The relevance of non-coding RNA sequences in human disease has increased remarkably over the past years. miRNAs represent the most extensively investigated category of ncRNAs in cancer since there are genetic and epigenetic defects causing their deregulation and contributing to tumorigenesis. However, other ncRNAs, such as PIWI-interacting RNAs (piRNAs), small nucleolar RNAs (snoRNAs), transcribed ultraconserved regions (T-UCRs) and large intergenic non-coding RNAs (lincRNAs) are emerging as key elements of cellular homeostasis. The deregulation of these RNAs may contribute to the development of many different human disorders, including cancer [14].

snoRNAs and scaRNAs play important roles in the maturation of rRNA, tRNA, snRNA as well as in mRNA biogenesis [34]. sno/scaRNAs may also be involved in human cancers as demonstrated by recent studies in MM, lymphomas and leukemias [17–22]. In this report we describe for the first time the global expression profiles of sno/scaRNAs in the cells from a large cohort of CLL cases already characterized for many features. These profiles were also compared with those of various sub-populations of normal B-cells from peripheral blood and from tonsils.

The identification of the normal B-cell counterpart of CLL (namely SM and MZ B-cells on one side and N B-cells on the other) is currently a debated question [35, 36]. Although based on a limited number of normal samples, our analysis revealed that the sno/scaRNA expression profile of leukemic cells is much more similar to N, MZ and M B-cells than to GC or total pB- cells. Therefore, sno/scaRNAs that significantly discriminate between CLL cells and N, MZ and SM B-cells, might be of relevance in disease pathogenesis. These are SNORA31, -6, -62, and 71C, all of them representing canonical “H/ACA snoRNAs”, which bind to conserved core box H/ACA snoRNP proteins, such as DKC1, GAR1, NHP2 and NOP10, and act mainly as guide RNAs for the site-specific pseudouridylation of specific target rRNA [15]. Notably, all of these ncRNAs were down-regulated in CLL cells (Figure 1B) irrespective of the presence or absence of other genetic lesions (data not shown). Specifically, SNORA31 was significantly down-regulated in association with its host gene TPT1 (Table 3), which encodes for a critical protein involved in the control of stemness, pluripotency, or tumor reversion [37]. In addition, TPT1 mRNA is capable of activating the dsRNA-dependent protein kinase PKR, which is in turn critical for the tumor suppressor function of TP53 [37]. At present it is unknown whether SNORA31 down-regulation may have a pathological role per se, or whether this down-regulation merely represents a marker of TPT1 down-regulation. SNORA6 and −62, were both down-regulated in association with their common host gene RPSA (Table 3). This gene encodes for a protein that, depending on its folding configuration, may have different cellular activities in specific compartments, that is the ribosomal protein SA or the laminin membrane receptor. Cytometric studies reported that the immature laminin receptor which, unlike the mature receptor, is not acylated, is specifically expressed on the surface of CLL B-cells but not in N, GC, or SM B-lymphocytes from normal tonsils. Moreover, its expression correlated with mutated IGHV status predicting a favorable prognosis in CLL [38]. These data are in apparent conflict with ours, although it is possible that down-regulation of the RPSA gene does not affect the translated gene fraction folded as immature laminin receptor, but rather the co-regulated expression of SNORA6 and −62. Finally, CLL cells significantly down-regulated SNORA71C located in a cluster at chromosome 20q11 including SNORA71A, -71B, and -71D.

Our data based on unsupervised analyses suggest an heterogeneous pattern of sno/scaRNA expression profiles within the major CLL subgroups classified according to biological, molecular and cytogenetic markers. This is different from the evidence in MM showing specific sno/scaRNA expression patterns associated with distinct molecular subgroups of the disease [19]. However, supervised analyses demonstrated specific, albeit limited, signatures of sno/scaRNA expression in distinct molecular and genetic CLL groups (Table 2). To note, SNORA70F was found consistently down-regulated in patients associated with adverse prognostic markers, such as unmutated IGHV, ZAP70 and CD38 positivity, 12+, and del11. SNORA70F is located within the first intron of the COBLL1 gene, the expression of which correlates significantly with that of SNORA70F in our dataset (Table 3). COBLL1 is down-regulated in UM-CLLs [39] as well as in CLL with a poor prognosis in general [40]. The exact function of the COBLL1-encoded protein is still unknown, although data have suggested an involvement in mid-brain neural tube closure [41]. Moreover, COBLL1 is a negative regulator of apoptosis in malignant mesothelioma cells and its expression is associated with a relatively better prognosis [42]. Finally, we provided evidence that patients with del11 or 12+ deregulated sno/scaRNAs located in the respective altered chromosome; in particular, 12+ samples exhibited a significant up-regulation of snoRNAs host genes as well (Table 2), supporting the notion that the gene dosage effects brought about by this lesion may have a pathogenetic value [43].

With regards to the potential clinical relevance of this specific ncRNA family in cancer, recent reports indicated the association of SNORD25, SNORD27, SNORD30, and SNORD31 with progression from smoldering to symptomatic MM [18] and the over-expression of SNORD71 in peripheral T-cell Lymphoma with favorable outcome [22]. In our study, we generated a 2-snoRNAs risk model which appears to be able to distinguish two different prognostic groups in our series of Binet stage A CLL patients, independently of all the other known molecular markers. Specifically, the high-risk group was characterized by the high expression of at least one of the two snoRNAs, SNORA74A and SNORD116-18.

Little is known about SNORA74A, which is found to be processed from the second intron of a long pre-mRNA-like transcript, termed precursor U19H RNA. At least five transcripts are obtained by alternative splicing of the long U19H gene, and only one form (approximately 2%) encodes for a protein, MATR3, involved in mRNA stabilization [44, 45]. This evidence may explain why SNORA74A expression does not correlate with that of MATR3, a phenomenon also observed in MM patients [19]. SNORD116-18 belongs to a cluster of 29 highly similar copies that, together with the SNORD115 cluster, are tandemly-arranged within the introns of the SNURF–SNRPN transcript, which contains at least 148 exons spanning more than 460 kb on chromosome 15q11. This genomic region is known to be affected by minimal deletions associated with the Prader–Willi syndrome (PWS) [46]. The expression of SNURF–SNRPN, as well as that of other several genes in this region, is finely regulated by a bipartite imprinting center (IC) which silences most maternal genes of the PWS critical region allowing the SNURF–SNRPN pre-mRNA to be expressed only from the paternal allele. However, mechanisms other than IC methylation may contribute to the deregulated expression of SNORD116 in MM [19]. To note, SNORD116-18 belongs to a subgroup of so-called “orphan” sno/scaRNAs which lack apparent complementarities to cellular RNAs. These molecules may play a role in the regulation of alternative splicing mRNAs, as demonstrated for murine SNORD115 which is processed to a shorter form binding to complementary target sequences on the HTR2C pre-mRNA for the correct alternative splicing of the serotonin receptor mRNA [47]. A role in the 3′ processing of selected snoRNAs has also been proposed for SCARNA22 which is deregulated in MM in association with its host gene MMSET, involved in the t(4,14) chromosomal translocation [17]. A similar function could be suggested for SNORD116 variants, as also predicted by the recent available snoTARGET open source [48]. In this perspective, it is conceivable that SNORD116-18 deregulation might also have a role in CLL cell since the involvement of uncorrected splicing mechanisms in CLL pathology is supported by increasing evidence [40, 49]. Unfortunately, the lack of either independent publicly available datasets or some standardizable methodology prevented the identified 2-snoRNA model from being considered a pure classifier; however, our results provided important indication on the possible role of non-coding RNA in the prognosis of CLL, and prompt for further investigations.

In conclusion, our data extend the current view of ncRNA deregulation in cancer pointing to the potential relevance of the sno/scaRNA family in the context of CLL which may contribute to discover novel putative molecular markers associated with the disease.

This work was supported by: Associazione Italiana Ricerca sul Cancro (AIRC) grant 5xmille no. 9980, 2010–15 to PT, AN, FM, MF, and MN, and AIRC IG10136 to A.N and IG10492 to M.F; Ministero Italiano dell’ Istruzione, Università e Ricerca (MIUR) (2009PKMYA2) to A.N. Recchia A.G. is supported by a grant from Fondazione ‘Amelia Scorza’ onlus, Cosenza. Colombo M is supported by AIRC grant to MF; Bossio S, Matis S and Massucco C are supported by a AIRC 5xmille grant.

Authors and Affiliations

1. Department of Clinical Sciences and Community Health, University of Milano, Milano, Italy

   Domenica Ronchetti, Laura Mosca, Sonia Fabris, Luca Agnelli, Gabriella Ciceri & Antonino Neri

2. SS Molecular Diagnostics, IRCCS S, Martino-IST, Genova, Italy

   Giovanna Cutrona

3. Department of Clinical Sciences and Community Health, University of Milan, Hematology 1 CTMO, Fondazione IRCCS Ca’ Granda Ospedale Maggiore Policlinico, F. Sforza, 35-20122, Milano, Italy

   Giacomo Tuana, Luca Agnelli & Antonino Neri

4. U.O.C. di Ematologia, Azienda Ospedaliera di Cosenza, Cosenza, Italy

   Massimo Gentile, Anna Grazia Recchia, Sabrina Bossio & Fortunato Morabito

5. Scientific Direction, IRCCS S Martino-IST, Genova, Italy

   Serena Matis, Carlotta Massucco, Monica Colombo & Manlio Ferrarini

6. Department of Pathology IRCCS S Martino-IST, Genova, Italy

   Daniele Reverberi

7. Department of Experimental and Clinical Medicine, University of Ferrara, Ferrara, Italy

   Massimo Negrini

8. Department of Experimental and Clinical Medicine, Magna Graecia University, Catanzaro, Italy

   Pierfrancesco Tassone

Corresponding author

Correspondence to Antonino Neri.

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

Contributions: DR analyzed the data, performed Q-RT-PCR, and wrote the manuscript; LM generated gene expression profiling data and analyzed the data; GT and LA performed statistical and integrative analyses; SF and GC performed FISH; SM, CM, MC, MG, SB, and GC performed the characterization of CLL samples for prognostic markers and cell purification; SM, CM, and DR performed B-cell subsets preparation and cell sorting; MN, FM, MF, AGR, and PT critically reviewed the manuscript; AN designed the study and wrote the manuscript. All authors approved the final version of the manuscript.

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