Introduction

Accumulating studies show that the tumour suppressor SOCS1 is one of the most frequently mutated genes in lymphomas, often affecting the coding sequence of SOCS1 protein. Depending on the type of mutation and lymphoma concerned, SOCS1 mutations have different impacts on progression-free and overall survival. Two antibodies binding the N- and C-terminals of SOCS1 would be a suitable “test pair” to identify truncated versions of SOCS1. We therefore compared the C-terminal antibody 424C with the N-terminal antibody 4H1.

Material and Methods

As 424C has already been characterised, we performed a comparative analysis of anti-SOCS1 antibody 4H1 using immunohistochemistry on human tonsil tissue and chamber slides, immunoblots on SOCS1 wildtype and mutated transfected HEK293 cells and lymphoma cell lines, and cross-reactivity analysis and epitope mapping with protein microarrays.

Results

Compared with 424C, anti-SOCS1 antibody 4H1 showed various cross-reactions with other proteins resulting in a “pancellular” immunohistochemical staining pattern in FFPE lymphoid tissue. Like 424C, 4H1 identified SOCS1 wildtype and SOCS1 mutations in immunoblot experiments but also bound an unknown protein with high intensity.

Conclusion

Anti-SOCS1 antibody 4H1 may be useful in a molecular setting, but is disqualified as an immunohistochemical diagnostic tool due to its very broad non-specific binding.