Included in the present study were 27 patients admitted to Department of Pediatrics with a clinical diagnosis of NS (independently of their mutational status and the presence of hematological anomalies). Three patients had a myeloproliferative disorder (NS/MPD), with monocytosis, atypical monocytoid cells, myelodysplastic features and granulocyte precursors in PB, thrombocytopenia and hepato-splenomegaly (2–6). Five patients with a diagnosis of JMML, fulfilling the EWOG-MDS criteria (8) were also studied. PB samples were collected in EDTA at diagnosis. Further blood samples were collected and analyzed in NS patients when hematological anomalies (e.g. anemia, thrombocytopenia, leukocytosis, splenomegaly, lymphadenopathy) and/or alterations of the functional pattern of circulating hematopoietic progenitors were observed. NS/MPD and JMML patients were evaluated at various stages during follow-up and treatment. Ethics committee approval and informed consent of the parents of the patients were obtained.

Genomic DNA was isolated from 200 μl of PB by the QIAamp DNA Blood Mini kit (Qiagen, Germantown, MD, USA). A molecular analysis of PTPN11, KRAS, SOS1, RAF1, BRAF, SHOC2, NRAS and CBL was performed as previously described (11–20).

Flow cytometric analysis was performed within 2 h after venipuncture. The absolute count of CD34⁺ cells and the apoptotic rate were evaluated by a three-color fluorescence for CD45, CD34 and Annexin V as follows. A total of 5×10⁵ nucleated cells were incubated for 20 min at 4°C with anti-CD34 PE (8G12; Becton-Dickinson, San José, CA, USA) and anti-CD45 PerCP (2D1; BD Biosciences, Franklin Lakes, NJ, USA). After incubation and red cell lysis by ammonium chloride, the samples were washed in cold phosphate-buffered saline (PBS) and incubated with Annexin V-fluorescein isothiocyanate (FITC) (Apoptosis Detection kit; R&D Systems, Minneapolis, MN, USA), according to the manufacturer’s instructions. The cells were then analyzed in a Coulter Epics XL2 (IL, Bedford, MA, USA) cytometer equipped with an argon laser. CD34⁺ cells were identified by a sequential gating strategy according to the ISHAGE protocol (26). Absolute CD34 counts were assessed by a two-platform method with a Sysmex K4500 counter (Sysmex Corporation, Kobe, Japan). At least 100 CD34⁺ cells were evaluated in each experiment.

Low-density mononuclear cells (2×10⁵) obtained from the patient PB by density centrifugation over Ficoll-Hypaque gradient were plated in multi well plates in 250 μl Iscove’s modified Dulbecco’s medium (IMDM) containing 30% fetal calf serum (FCS) (both from Sigma-Aldrich, St. Louis, MO, USA), 0.3% noble agar and 100 U/ml rhIL-3 and decreasing concentrations (20, 10, 5, 1, 0.1 ng/ml) of rhGM-CSF (both from Invitrogen Life Technologies, Carlsbad, CA, USA). After 14 days, single aggregates of >40 cells were scored as CFU-GMs. GM-CFU assay was also performed without GM-CSF stimulation. GM-CFU assay in the same culture conditions was also performed in 21 pediatric controls (median age, 9.0; range, 1–18 years).

The patients were divided into 3 groups: NS, NS/MPD and JMML. Historical controls (n=68) from our laboratory were utilized for the absolute count of CD34⁺ in PB and the apoptotic rate (25).

For the absolute count of CD34⁺ cells and apoptotic rate, the values for each patient were compared with the mean control value adjusted for age, as previously published (25).

The cell culture data and the absolute count of CD34⁺ cells and the apoptotic rate results were analyzed using the non-parametric Kruskal-Wallis test. Pairwise comparisons for the disease groups were performed for each of the GM-CSF concentration utilized in the cell cultures, as well as for the 4 variables analyzed in the test (absolute CD34⁺, percentage of CD34⁺/Annexin V⁺, absolute CD34⁺ to the mean age group value ratio, percentage of CD34⁺/Annexin V⁺ to the mean age group value ratio). Fisher’s exact probability test was utilized for correlations between the groups.

The mutational spectrum of our series of NS, NS/MPD and JMML patients is shown in Table I.

All JMML patients showed monocytosis >1,000/μl. Ten out of the 27 NS patients showed monocytosis >1,000/μl, which included the 3 NS/MPD patients (Tables I and II).

All JMML patients showed thrombocytopenia as well as 1 out of the 3 NS/MPD patients. In the other NS patients, the platelet counts were in the range of normality, without a correlation with monocyte counts (R=0.016) (Table I).

The PB absolute CD34⁺ cell counts and apoptotic rates in the different groups of patients are shown in Tables I and II. In JMML and NS/MPD patients, we observed high levels of circulating CD34⁺ cells with a low apoptotic rate. In NS patients, CD34⁺ cell counts were normal, whereas their apoptotic rate was significantly lower than that in the controls (p<0.01). Concerning the absolute CD34⁺cell count, statistically significant differences were noted among the NS and JMML (p=0.001), NS and NS/MPD (p<0.05), controls and JMML (p<0.01), and controls and NS/MPD patients (p<0.05). In contrast, no differences in the absolute CD34⁺ cell count were observed between the controls and NS or between the NS/MPD and JMML patients. Normalizing the absolute CD34⁺cell count for age (absolute CD34⁺ to mean age group value ratio), the results from the pairwise comparison did not change.

A pairwise comparison of the Annexin V⁺ percentage showed a statistically significant decrease in the apoptotic rate in each disease group when compared with the controls: NS (p<0.01), NS/MPD (p<0.05), JMML(p<0.01); whereas no significant difference was observed between NS/MPD and JMML, JMML and NS, and NS/MPD and NS patients. When the percentage of Annexin V⁺ cells was normalized for age (percentage of Annexin V⁺/CD34⁺ cells to mean age group value ratio), the results for the pairwise comparison did not change.

In the JMML patients, the clonogenic assays from PB showed hypersensitivity to GM-CSF and spontaneous CFU-GM growth (except in one patient previously treated with chemotherapy at another center who did not show spontaneous CFU-GM growth) (Table I). In 3 out of 3 NS/MPD patients we observed hypersensitivity to GM-CSF (in patient NS/MPD3 during the follow-up) and in 2 out of 3 spontaneous CFU-GM growth was noted. In 2 NS patients (NS13 and NS19) we observed hypersensitivity to GM-CSF, and no spontaneous CFU-GM growth. One NS patient (NS11) showed hypersensitivity to GM-CSF and spontaneous CFU-GM growth. This patient had a favorable clinical outcome, and the clonogenic assays performed 6 months later showed normal results.

We observed a significant difference in the distribution and in the median values of CFU-GM among the 3 groups (JMML, NS, NS/MPD) (Table II). Table III (pairwise comparisons of GM-CSF-stimulated clonogenic assays) showed that at different GM-CSF concentrations, JMML patients were significantly more responsive to GM-CSF than both the controls and NS patients. Concerning unstimulated cultures, a significant growth advantage was observed also in NS/MPD when compared with the controls and NS patients (Table III). Specifically, clonogenic assays without GM-CSF were able to distinguish between NS and NS/MPD patients. Fisher’s exact probability test showed a significant correlation between the groups in the unstimulated colony growth tests (0% in controls, 4.2% in NS, 80% in JMML, 66.7% in NS/MPD, p<0.001).

Six NS patients showed isolated monocytosis >1,000/μl, 2 NS patients showed isolated hyper-responses to GM-CSF, 5 NS patients showed an isolated increase in circulating CD34⁺ cells. In all of these patients a 12-month follow-up showed no alterations in clinical findings. Patients NS11 and NS/MPD1 showed monocytosis >1,000/μl, a hyper-response to GM-CSF, CFU-GM growth without GM-CSF stimulation, high circulating CD34⁺ counts with a low apoptotic rate. In these 2 NS patients a clinical and laboratory follow-up was performed. Patient NS11 carrying the Glu76Asp PTPN11 mutation, was phenotypically characterized by polyhydramnios in the prenatal history, typical facial dysmorphisms, pulmonic stenosis, bilateral cryptorchidism and normal neuropsychomotor development. His clinical follow-up in the following months was normal, and a laboratory hematologic evaluation performed 12 months later showed normal response to GM-CSF, no spontaneous colony growth and normal CD34⁺ cell and monocyte counts.

Patient NS/MPD1 was first evaluated at the age of 2 months while she was in the cardiac surgery unit due to obstructive hypertrophic cardiomyopathy. A clinical diagnosis of NS was confirmed by the molecular analysis of the PTPN11 gene, that revealed the Phe285Ser mutation. A preliminary hematological evaluation evidenced only mild hepatomegaly and monocytosis. Clonogenic assays and flow cytometry showed hypersensitivity to GM-CSF, spontaneous CFU-GM growth, increased circulating CD34⁺ cells with a low apoptotic rate. At the age of 12 months, the patient showed splenomegaly, thrombocytopenia and monocytosis, with the presence in the peripheral blood smear of 10% of atypical monocytoid cells, moderate myelodysplastic features and granulocyte precursors. Bone marrow aspirate showed mild myelodysplasia and the presence of 15% of atypical monocytoid elements. A polymerase chain reaction (PCR) for bcr/abl rearrangement was negative. The HUMARA assay performed on peripheral blood populations was normal, excluding a frank JMML evolution and suggesting a polyclonal myeloproliferative disorder, described in NS (2). Hence, a diagnosis of NS/MPD was made. Thrombocytopenia and splenomegaly persisted over the following months, and the clinical course worsened, with a progressive development of lymphatic dysplasia with thoracic duct ectasia, progressive severe respiratory insufficiency, pleural effusion and exitus at the age of 20 months for acute cardiopulmonary failure.

Patients NS/MPD2 and NS/MPD3 were diagnosed in the first month of life presenting a myeloproliferative disorder. Table IV shows the clinical and laboratory follow-up of the NS/MPD patients, and Fig. 1 shows a detailed follow-up of patient NS/MPD1.