The search for tumor-specific antigens (TSAs) has considerably accelerated during the past decade due to the improvement of proteogenomic detection methods. This provides new opportunities for the development of novel antitumoral immunotherapies to mount an efficient T cell response against one or multiple types of tumors. While the identification of mutated antigens originating from coding exons has provided relatively few TSA candidates, the possibility of enlarging the repertoire of targetable TSAs by looking at antigens arising from non-canonical open reading frames opens up interesting avenues for cancer immunotherapy. In this review, we outline the potential sources of TSAs and the mechanisms responsible for their expression strictly in cancer cells. In line with the heterogeneity of cancer, we propose that discrete families of TSAs may be enriched in specific cancer types.
Current protocols used to extract and purify histones
are notoriously
tedious, especially when using yeast cells. Here, we describe the
use of a simple filter-aided sample preparation approach enabling
histone extraction from yeast and mammalian cells using acidified
ethanol, which not only improves extraction but also inactivates histone-modifying
enzymes. We show that our improved method prevents N-terminal clipping
of H3, an artifact frequently observed in yeast cells using standard
histone extraction protocols. Our method is scalable and provides
efficient recovery of histones when extracts are prepared from as
few as two million yeast cells. We further demonstrate the application
of this approach for the analysis of histone modifications in fungal
clinical isolates available in a limited quantity. Compared with standard
protocols, our method enables the study of histones and their modifications
in a faster, simpler, and more robust manner.
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