CSF is mainly produced at the choroid plexus, where it is separated by blood circulation through the blood–CSF barrier. Linsitinib supplier It is produced at a flow-rate of approximately 500 mL/24 h [80] and its composition is strictly regulated by the selectivity of the BBB [79]. The CSF proteome is
for its most part (80%) composed of proteins derived from blood and, as in plasma, albumin and immunoglobulins represent approximately 70% of the total amount of CSF protein [81]. The remaining 20% of CSF proteins are produced in the brain, although they are rarely considered brain specific [80] and [82]. Since late stage HAT is characterized by a meningo-encephalitis [14] and [83] and that CSF examination is part of the current diagnostic workflow, the reasoning for looking for novel disease progression markers in this body fluid seems pertinent. Alterations in the protein content of CSF are of particular clinical utility for this website many neurological disorders. An increased protein concentration can be indicative of either a BBB dysfunction or an increased intrathecal synthesis of proteins.
The quotients of albumin (QAlb) and immunoglobulin (QIg) are used to evaluate and quantify this dysfunction [79], [80] and [82], and the latter can be particularly helpful to indicate an inflammatory process occurring in the brain [82] and [84]. The increased concentration of immunoglobulins in the CSF of late stage HAT patients, with IgM being the predominant class, has been known since the 1980s [85]. This observation agrees with the absence of the switch between IgM and IgG, and the low decay of CSF antibodies characteristic of
the humoral immune response in the brain [82]. More recently, it has been demonstrated that an increased fraction of IgM of intrathecal origin in S2 HAT patients [73] and [86] is indicative of the presence of a brain inflammatory Morin Hydrate process not associated to damage of the BBB. IgM, and in particular those of intrathecal origin, are currently considered as the best alternative to a WBC count for staging T. b. gambiense HAT. A rapid agglutination test for the evaluation of IgM concentration in CSF has been developed (Latex/IgM) and a high correlation between the final Latex/IgM titer and intrathecal IgM production has been shown [87] and [88]. Despite this method has high accuracy for stage determination [88], strong enough evidence to support its introduction into clinical practice is still missing. Moreover, Latex/IgM exhibited limited utility for the evaluation of outcomes after treatment. Indeed, Latex/IgM combined with a WBC count accurately detected relapses at 18 months after treatment, but IgM normalized very slowly over time in cured patients [89] and [90].