Salivary epidermal growth factor correlates with hospitalization length in rotavirus infection

Rotavirus (RV) infection is the most common cause of severe diarrhoea in children and may cause serious dehydration that usually requires hospitalization [1]. Predominantly, but not exclusively, RV infects the terminally differentiated enterocytes in the small intestine and it induces mucosal damage, villus atrophy and necrosis of epithelial cells [2]. RV infection alters the function of the small intestinal epithelium, resulting in characteristic diarrhoea, secondary to enterocyte destruction.

There are currently not reliable specific biomarkers for RV infection. Identifying new correlates of disease activity may help in designing new treatments and more efficacious RV vaccines. Use of saliva as a proxy indicator of intestinal immunity has been proposed as a non-invasive source of biomarkers [3]. Salivary IgA has been recently suggested as a correlate for protection for norovirus intestinal infection [4].

In a recent whole blood transcriptomic analysis of RV-infected patients, we reported a 23.7 fold increase in the expression of the IFI27 gene, an interferon-related gene with unknown function in the RV infection [5]. Moreover, this gene has recently been associated to the epidermal growth factor (EGF) and involved in proliferation of epithelia [6]. EGF, also known as epithelial growth factor, is a single chain polypeptide secreted by the submandibular salivary glands and other exocrine intestinal glands. In vivo actions of EGF in the gastrointestinal tract include promoting wound healing and tissue repair, inducing epithelium proliferation and promoting differentiation [7]. A significant contribution of salivary EGF to the maintenance of the integrity of the oesophageal mucosa has been demonstrated in experimental and clinical settings [8]. Patients with low salivary EGF levels are predisposed to severe oesophageal damage by gastro-oesophageal reflux [9].

The aim of the present study was to measure the levels of EGF in saliva from acute-phase RV-infected children and to assess its potential relationship with disease course and severity.

Patients in the RV-infected group ranged in age from 1 to 40 months (median of 12.5 months) at recruitment. Healthy control children ranged in age from 6 to 7 months (median of 7 months). Demographic and clinical characteristics are summarized in Tables 1 and 2.

Median levels for EGF in saliva from acute-phase RV-infected patients were 777 (SD = 529) pg/ml. Salivary EGF levels where significantly lower in convalescent patients (356 pg/ml; SD = 242; Wilconxon test, P-value = 0.015) and healthy controls (337 pg/ml; SD = 119; Wilconxon test, P-value = 0.001474); Fig. 1a. These variations in EGF levels were not age-related (Fig. 1b).

When assessing possible correlations between EGF levels and clinical variables in RV infected subjects, a significant negative correlation was found between salivary EGF concentration and length of hospital stay (P-value = 0.022; r ²  = −0.63). We did not find any other significant association between EGF levels and other clinical parameters of disease (Fig. 1c).

In a previous whole blood transcriptomic analysis [5] carried out in RV-infected patients vs control children, a remarkable over-expression of IFI27 gene was reported. IFI27 belongs to the family of interferon inducible genes, and recently it has been associated to epidermal proliferation and EGF [6]. In addition, IFI27 was previously identified as a marker of epithelial cancers and psoriatic lesions [10] and related to systemic lupus erythematosus (SLE) [11]. However, the exact role of IFI27 in the RV infection physiopathology is still unknown, although based on our results we can suggest that RV infection might activate an interferon-mediated mechanism of mucosal recovery after infection damage through a pathway mediated by IFI27. The observed association between IFI27 expression and EGF requires a more in-depth analysis, and the mechanistic approach needs to be clarified.

EGF is linked to epithelia regeneration after mucosal lesions, promoting mucosal wound healing and tissue repair [12]. Previous studies in neonatal pigs infected with RV already pointed to a beneficial role of high physiological levels of EGF in stimulating recovery of epithelium in the small intestine following infection [13]. EGF application in the mucosa can promote intestinal proliferation and improve restoration after intestinal injury, and it might be an effective treatment against intestinal ischemia-reperfusion injury in rats [14]. The hypothesis of EGF supplementation after intestinal injury as a potential treatment for improving outcome in patients has been put forward by other authors based on animal studies [15]. This finding might lay the ground for a new recovery treatment after RV infection.

Our present study shows that salivary levels of EGF are increased during natural RV infection and that they may correlate with the severity of the disease in terms of length of hospital stay. The over-expression of EGF levels in infected patients might suggest a host recovery response to the damage induced by RV in the intestinal mucosa. The disruption in the normal homeostasis of mucosa would induce the production of EGF, also expressed in the submandibular salivary glands, in order to restore the integrity of mucosa after infection.

Interestingly, we found that the higher the levels of EGF in acute-phase samples from RV-infected patients upon admission, the shorter the length of stay in hospital. It could be argued that the greater level of EGF reflects a more powerful response of mucosal homeostasis, thus facilitating a faster recovery, and a reduction in the length of hospitalization. This association, if prospectively confirmed, might allow to make predictions on recovery of mucosal integrity and hospitalization length with a simple and non-invasive methodology. The use of saliva as a non-invasive proxy for intestinal immunity after enteric infection opens the door to the search for new specific biomarkers for RV infection that might correlate with clinical parameters of disease.

One limitation of the present study is the limited number of individual analysed, however the novelty of our findings merits consideration and further confirmatory studies. Another limitation derives from the different localization of previous gene expression analyses (performed in whole blood), and our EGF quantification (performed in the epithelial mucosa).