2011
DOI: 10.1128/iai.00338-10
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Leukocytes Infiltrate the Skin and Draining Lymph Nodes in Response to the ProtozoanLeishmania infantum chagasi

Abstract: The vector-borne protozoan Leishmania infantum chagasi causes minimal inflammation after inoculation into skin but disseminates to cause fatal visceral leishmaniasis. To define the inflammatory response at the parasite inoculation site, we introduced metacyclic L. infantum chagasi promastigotes intradermally into BALB/c mouse ears and studied inflammatory cells over 7 days. Ly6G؉ neutrophils rapidly infiltrated the dermis, peaking after 6 to 24 h. Macrophages and NK cells next infiltrated the dermis, and NK fo… Show more

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Cited by 87 publications
(115 citation statements)
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“…survive inside macrophages throughout chronic infection of their mammalian hosts [3]. Reports over the past 5 years have made it clear that neutrophils are among first cells to arrive at the site of a sand fly bite and to take up the parasite [5,6]. An essential step in our understanding of the role of PMNs in leishmaniasis is the bidirectional effect of parasites on neutrophils and vice versa.…”
Section: Discussionmentioning
confidence: 99%
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“…survive inside macrophages throughout chronic infection of their mammalian hosts [3]. Reports over the past 5 years have made it clear that neutrophils are among first cells to arrive at the site of a sand fly bite and to take up the parasite [5,6]. An essential step in our understanding of the role of PMNs in leishmaniasis is the bidirectional effect of parasites on neutrophils and vice versa.…”
Section: Discussionmentioning
confidence: 99%
“…One thing that is clear is that neutrophils are abundant and interact extensively with the parasite during the first hours of infection [5,6,19]. Many other diseases such as those causing lung inflammation [43] or autoimmune disorders [44] document a role for highly activated neutrophils contributing to off-target cellular pathology.…”
Section: Discussionmentioning
confidence: 99%
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“…On the basis of these considerations, there is a strong need to develop appropriate screening technologies. The use of fluorescent reporter genes such as those coding for green fluorescent protein (GFP) (17)(18)(19) and the red versions red fluorescent protein (RFP) (20,21) and mCherry (21,22) have considerably facilitated the screening and testing of antimicrobial agents against axenic amastigotes and intracellular amastigotes, allowing both in vitro and real-time visualization in vivo. Although animal models are well established for large-scale primary drug screening, its practical use is limited due to high costs.…”
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confidence: 99%