This immunological function induced by cells within the LN is an extensive area of research. To clarify the general function of LN, to identify cell populations within the lymphatic system and to describe the regeneration of the lymph vessels, the experimental surgical
technique of LN dissection has been established in various animal models. In this review different research areas in which LN dissection is used as an experimental tool will be highlighted. These include regeneration studies, immunological analysis and studies with clinical questions. LN were dissected in order to analyse the different cell subsets of the incoming lymph in detail. Furthermore, LN were identified as the place where the induction of an antigen-specific response occurs and, more significantly, where this immune response is regulated. During bacterial infection LN, as a filter of the lymph system, play a life-saving role. In addition, LN are essential for the see more induction of tolerance against harmless antigens, because tolerance could not be induced in LN-resected animals. Thus, the technique of LN dissection is an excellent and simple method to identify the important role of LN in immune responses, tolerance and infection. The lymphoid system consists of three different types of lymphoid
tissues: primary, secondary and tertiary lymphoid. The primary lymphoid organs are the bone marrow (BM) and thymus, and the secondary lymphoid organs include the spleen, Peyer’s patches (PP) and lymph nodes (LN). Tertiary lymphoid tissues selleckchem develop
during inflammation and are therefore highly variable structures. As this review focuses on LN dissection, find more all other lymphoid tissue structures will not be mentioned further (for more details see [1]). In mammals, LN are located all over the body. They all have the same architecture and are populated by the same cell types (Fig. 1). Their function is to filter the lymph coming from the draining area and to scan the lymph for antigens. Either an immune response to pathogenic antigens is initiated or, in the case of harmless antigens, tolerance [2]. In brief, antigen-loaded dendritic cells (DC), coming from the draining area via the afferent lymphatics, present their antigens to T lymphocytes in the T cell area or the paracortex. T cells which are T cell receptor-specific for the presented antigens are activated; they differentiate and proliferate. T helper cells, one class of activated T lymphocytes, migrate into the B cell area or cortex to assist B cells. These antigen-specific B cells differentiate into plasma cells for effective antibody production. All activated effector cells, such as plasma cells, CD4+ or CD8+ T cells, migrate to the medulla, where they leave the LN via efferent lymphatics or the blood system to travel to the inflamed or endangered area of their specific draining area. This precise migration is possible because of homing molecules which are up-regulated on effector cells after activation.