This may explain why high-frequency clones are shared between ind

This may explain why high-frequency clones are shared between individuals, and might be a plausible explanation for ‘public’ T-cell clones.10,22,39 This phenomenon describes a situation in which the same TCR sequence is produced in different individuals, as a response to identical antigen presentation. Findings also show that public TCRs can sometimes be found within individuals

www.selleckchem.com/products/gsk2126458.html sharing a common MHC allele, for example, in response to infectious diseases.10,39 This aspect of the repertoire may have serious implications for our understanding of the initial ability of an individual to fight incoming threats. Biases in TCRs have also been observed in cancer, autoimmune diseases and in responses to allergens.39 Although these public T-cell responses against specific pathogens

may provide a first line of defence, they may have a weakness in the rapid response to RNA viruses, which mutate rapidly, such as HIV and its simian counterpart.40 A completely different and novel approach to characterize the receptor repertoire is by network analysis. Many structural features can be studied from the aspect of network architecture, and so might help to better understand the dynamics of the immune click here response. Extended analysis of the zebrafish B-cell repertoire was performed by the construction of sequence and mutation networks.41 This analysis revealed that the fish sequence population self-organizes into two distinct groups, based on their network structure and their V–J combinations usage. The first group shows a uniform V–J combination

utilization with a uniformly connected network, whereas the other group revealed distinct subsets of immunoglobulin sequences, in the form of a much highly connected sub-network and higher V–J combination frequencies. A plausible hypothesis Erastin research buy is that this second group underwent a more complex immune response whereas the first one might only have responded to a minor challenge. The enormous quantity of reads generated by NGS technologies necessitates cautious interpretation. Potential errors during the sequencing process may skew interpretation. Therefore, repertoire analysis reliability depends on sequencing depth and coverage, but also on sequencing accuracy. Nguyen et al.42 recently tried to directly assess these error rates and proposed new approaches to reduce the number of erroneous sequences within the repertoire by profiling these errors and implementing quality filters. For this, they analysed specific transgenic TCRs obtained from RAG-deficient mice, allowing them to express a single germline rearranged TCR and therefore to compare the sequenced receptor with the original DNA. Their findings showed a total rate of 1–6% erroneous sequences, which are greatly, but not totally, reduced after the filtering process.

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