Association of serum TNF-α, IL-8 and free light chain with HLA-DR B alleles expression in pulmonary and extra-pulmonary sarcoidosis

In this study we investigated whether HLA-DRB * sub-typing could distinguish between sarcoidosis patients with pulmonary or extra-pulmonary involvement. We found that among the 16 HLA DRB alleles only *7 and *12 were different between sarcoidosis patients and controls with *12 being identified as a risk factor for sarcoidosis [45]. This study shows also a significant difference between the overall distribution of the HLA-DRB1 alleles between pulmonary sarcoidosis patients and patients with EPS. We further demonstrated increased levels of serum TNF-α and IL-8 in pulmonary sarcoidosis patients, while TNF-α was not increased in EPS subjects. Serum levels of FLCs were higher in EPS patients and not in pulmonary sarcoidosis. This is the first report showing different expression of HLA-DRB sub-types in pulmonary and EPS. The differential presence of pro-inflammatory markers such as TNF-α, IL-8, and FLCs may point to a different pathology in the two sarcoidosis subgroups.

Among the alleles tested, only the expression of the *07 and *12 were significantly altered in sarcoidosis with the frequency of *07 being decreased whereas that of *12 being increased compared with control subjects. It has previously been reported that the presence of the HLA-DR B *7 allele is related to a good disease prognosis [46,47]. Indeed, our patients with this genotype had good response to treatment. In contrast, in Swedish sarcoidosis patients the levels of DHL-DR *7 are increased [48]. The frequency of HLA-DR B*012 expression has been extensively reviewed [49] and the HLA DR-B*12 frequency is similar in our population as in three other populations from UK, Holland and Japan.

Variations in HLA-DRs associations have also been reported in sarcoidosis patients across different ethnic groups. For example, although the frequency of HLA-DRw52 was significantly greater in Japanese sarcoidosis patients compared to control groups there was no significant association with HLA-B antigens [50]. In addition, an association between sarcoidosis and HLA-DR5 has been reported in a German cohort of sarcoidosis patients [51]. This emphasizes that there may be ethnic differences in the expression of these specific alleles in sarcoidosis patients and that there is a need to further analyze other HLA class I and II subtypes in Iranian sarcoidosis patients in future studies.

We also report enhanced levels of serum IL-8 in both pulmonary sarcoidosis and EPS patients. To our knowledge there has only been one previous report showing elevated IL-8 levels in sarcoidosis [52]. Car and colleagues showed that IL-8 levels were significantly increased in bronchoalveolar fluid (BAL) of patients with sarcoidosis [53]. IL-8 is rapidly produced by different cell types upon exposure to inflammatory stimuli such as TNF-α and LPS and is considered as one of the most potent neutrophil chemoattractants in human tissue [54-57]. Recent evidence using blood transcriptomic analysis [58] indicates that neutrophilia is present in sarcoidosis patients as well as in other interferon- and immune-related diseases linked to activation of pattern recognition receptors and to anti-bacterial and -viral defenses. The clinical importance of the increased levels of IL-8 in serum and BAL needs further testing.

In addition, serum levels of TNF-α were increased in patients with pulmonary sarcoidosis but not in those with EPS. TNF-α is a pro-inflammatory cytokine previously shown to play a critical role in the pathogenesis of Th1 responses and to be elevated in sarcoidosis patients [58]. TNF-α plays a significant role in antigen-stimulated, cell-mediated immune responses and in the development of non-caseating granulomas in a variety of diseases [59]. In sarcoidosis, alveolar macrophage-derived TNF-α participates in the induction and maintenance of granulomas [60] and high levels of TNF-α released from alveolar macrophages seem to correlate with disease progression [61]. In addition, BAL levels of TNF-α and IL-6 are significantly higher in pulmonary sarcoidosis patients compared with control subjects [62]. Thus, we were able to recapitulate the BAL findings in relation to TNF-α in blood in our study.

However, the failure to demonstrate increased serum levels of IL-1β and IL-6 in sarcoidosis requires further investigation. This may result from the involvement of distinct cell types present in blood and BAL since these cytokines and chemokines are all stimulated by the same stimuli involving NF-κB activation [63]. This may also explain the differences in TNF-α expression observed between pulmonary sarcoidosis and EPS.

We also report elevated levels of both κ and λ FLC in the serum of EPS patients but not patients with pulmonary sarcoidosis. Sarcoidosis is known as a T cell mediated disease but B-cells may play a role in its pathogenesis particularly in chronic disease [64,65]. It is possible that the release of free light chains is from a distinct set of inflammatory cells in the blood of these patients. A growing body of evidence suggests that serum FLCs could be useful biomarkers in several immunological conditions as they reflect B-cell polyclonal activation including active sarcoidosis [65]. Serum FLC levels are also elevated in lupus [66], rheumatoid arthritis and Sjögren syndrome [37,45,67] where they are also associated with the active state of the disease. Serum FLCs have also recently been reported as biomarkers of systemic sclerosis activity and severity [68,69]. In the current study the expression of κ and λ FLCs was greater in EPS patients compared with patients with pulmonary sarcoidosis. The differential expression of κ and λ FLCs in EPS and pulmonary sarcoidosis requires confirmation in other cohorts and its functional importance needs to be further established. However, we speculate that B cells may play a more significant role in EPS compared to pulmonary sarcoidosis and that these patients may benefit from B cell-directed therapy.

In conclusion, we report for the first time that HLA DRB *12 may be indicative of sarcoidosis and that there is a differential HLA DRB allele usage between patients with EPS and pulmonary sarcoidosis. There were also differences in serum inflammatory markers between these two groups of sarcoidosis patients with patients with pulmonary sarcoidosis having greater levels of TNF-α and IL-8 than EPS and control subjects. Conversely, the expression of κ and λ FLCs was greater in EPS patients compared with pulmonary sarcoidosis patients. Overall, we report a link between HLA-DRB sub-types and inflammation in Iranian patients with sarcoidosis. We suggest that these novel markers should be readily incorporated into current laboratory analysis as they are relatively cheap and rapid, taking less than 48 h, and provide additional parameters for the differentiation of subtypes of sarcoidosis.