Follow-up evaluation of the immunological status of children admitted for acute cerebral nervous system infections: a retrospective study

We enrolled patients admitted to the Bambino Gesù Children Hospital, Roma, Italy, between 1st January 2006 and 30th June 2016 with the following diagnosis of ACNS infection: meningitis, meningoencephalitis, encephalitis and cerebellitis. We included all patients younger than 18 years. Exclusion criteria for selection were varicella-zoster virus infection and any of the following comorbidities: neurological disorders, chronic diseases, malignancy, known acquired or congenital immunodeficiency and/or immunosuppressive therapy. All patients underwent at least one follow-up evaluation to check clinical, vaccination and immunological status. To avoid bias due to possible effects of the recent disease, immunological exams were performed at least 1 month after the acute phase. At the follow-up evaluation, all patients were in good clinical condition, without either fever or other acute symptoms.

In details, laboratory tests included measurement of: serum antibodies against vaccine antigens; serum levels of Immunoglobulin (Ig) M, G, and A; complement levels; lymphocyte subpopulations; proliferation and differentiation of B cells. Serum antibodies against vaccine antigens, namely tetanus, HI, SP, Bordetella pertussis and Hepatitis B virus and serum levels of IgM, IgA and IgG were measured using a commercial ELISA kit for each antigen (Binding Site) and an in-house ELISA respectively. Coating of plates was carried out with an anti-IgM/IgG/IgA (Cat #109-006-064). Peroxidase-conjugated anti-IgM (cat #109-36-129), anti-IgG (cat #109-036-008), or anti-IgA (cat #109-036-011) (all from Jackson Immunoresearch) were used as primary antibodies. Purified serum IgG and IgA, and IgM purified from a myeloma cell line (Jackson Immunoresearch) were used as standards. Peripheral blood mononuclear cells (PBMCs) were isolated from blood on density gradient centrifugation (Lympholyte, CEDARLANE). PBMCs were loaded with CFSE (Life Technologies) to track divided cells. Briefly, 1 × 10⁶ cells /mL were resuspended in PBS 1% FCS and loaded with 1 μM CFSE for 20 min at 37 °C. Cells were then stimulated with 0.25 μM CpG-B ODN2006 (Hycult Biotech). Flow cytometry was then conducted to count the lymphocyte subpopulations and to evaluate proliferation and differentiation of B cells (CD3, CD4, CD8, CD19, CD24, CD38, IgM, CD16/56). Cells were stained with the appropriate combination of fluorochrome-conjugated antibodies, according to standard techniques. Dead cells were excluded from analysis by side/forward scatter gating. At least 50,000 events gated on living cells were analysed, whenever possible, for each sample. Samples were acquired on a BD Fortessa X-20.

The following four criteria were considered diagnostic for immunological alteration: absence of antibodies against vaccine antigens; age-related reduction of immunoglobulin values; reduction of B cell populations, namely memory B cells; defective proliferation and differentiation of B cells.

R, version 3.2.3 (R Foundation for Statistical Computing, Vienna, Austria. http://​www.​R-project.​org/​) was used for data analysis. We compared the laboratory results of our patients with age-matched normal values [13, 14]. The t-test was used for comparison of means of Ig and lymphocyte subclass counts. A p value less than 0.05 was considered significant.