Coxiella burnetii Avoids Macrophage Phagocytosis by Interfering with
Coxiella burnetii Avoids Macrophage Phagocytosis by Interfering with Spatial Distribution of Complement Receptor 3 By Lionel Williamson
Introduction Coxiella burnetii is an obligate intracellular bacteria l Its survival strategy in monocytes/ macrophages is based on growth in acidic phagosomes that do not fuse with lysosomes l Infection of humans usually occurs by inhalation of these organisms from air that contains airborne barnyard dust contaminated by dried placental material, birth fluids, and excreta of infected herd animals l
Introduction It causes Q fever In 1999, Q fever became a reportable disease in the United States l Most acute cases of Q fever begin with sudden onset of one or more of the following: high fevers (up to 104 -105° F), severe headache, general malaise and myalgia, confusion, sore throat, chills, sweats, non-productive cough, nausea, vomiting, diarrhea, abdominal pain, and chest pain l As many as 65% of persons with chronic Q fever may die of the disease. l l
Overview of paper critical part of infection is C. burnetii getting into the monocyte l Difference between virulent and avirulent strains is this ability to survive in the monocyte l The
Key terms l Complement receptor 3 (CD 11 b: CD 18) binds to a pathogen surface that has been opsonized with complement and promotes pathogen phagocytosis l CD- cluster of differentiation l Integrin are heterodimeric cell surface proteins involved in cell-cell and cell-matrix interactions they are involved in adhesive interactions and ligand binding
Key terms l RANTES- is a chemokine that stimulates the migration and activation of cells especially phagocytic cells. It induced psuedopodal extensions that expressed CR 3 In THP-1 cells l HIV-1 Nef also acts like a chemokine stimulating migration inside the phagocyte. Same as above
What did they know l They knew that uptake of the avirulent strain was mediated by άβ integrin and CR 3 l Virulent strain entered the monocyte through άβ integrin but interfered with the CR 3 which appeared to prevent phagocytosis
What did they know l CR 3 must be activated to promote ligand binding and phagocytosis l Activation required signals from other integrins, chemoattractant receptors or LPS receptors l Ex. ligation of άβ integrin and integrin associated protein (IAP) enhances CR 3 binding
What did they know CR 3 clustering is correlated to increased binding and phagocytosis (Immobile form) l The switch from an inactive to an active form is associated with an alteration in the mechanism of interaction CR 3 with the cytoskeleton l An immobile subset of CR 3 linked to the cytoskeleton is more efficient for phagocytosis than freely diffusing receptors l
What did they know l F- actin is part of the cytoskeleton infrastructure l The virulent but not the avirulent strain has the ability to reorganize the F-actin in THP-1 monocytes l They hypothesized that C. burnetii mediated impairment of CR 3 activity may result from effects of actin reorganization
Receptor distribution in C. burnetiistimulated monocytes l THP-1 monocytes were tagged with m. Ab directed to monocyte receptors involved in C. burnetii recognition l Large beads coated with anti mouse Ig. G Abs and F-actin labeling l Also beads were attached to monocytes tagged with m. Ab directed CD 11 b, CD 18, άβ integrin, IAP (no bead phagocytosis was observed)
Exp. cont l THP-1 were stimulated with virulent C. burnetii l The stimulation caused F-actin reorganization and psuedopodal extensions in 60% and 40% did not change l In the 40% beads bound to Cd 11 b and CD 18, άβ integrin, and IAP were bound randomly as in the control cells
cont l l In the 60% all the beads attached to CD 11 and CD 18 were found outside the deformation area This response was seen in as early as 10 min and continued for about 60 min In contrast the beads bound to άβ integrin were present at the leading edge of the protrusion (1/4 of άβ integrin was found on the protrusion) The pattern of IAP was similar to the integrin
cont
cont TO prove that the lack of CR 3 on the protrusion was not caused by the size of the beads they did the experiment using smaller beads l They were able to detect CR 3 on the protrusions in <10% compared to 25% of άβ integrin, and IAP were detected on the protrusions l Confirmed that CR 3 was excluded from the extensions l
cont
Cont l They repeated the experiment with circulating monocytes with the same results l Avirulent strain did not induce psuedopodal extension or F-actin reorganization and as a consequence the distribution of CD 11 b, CD 18, άβ integrin, and IAP was similar to control cells
Receptor distribution in RANTESstimulated monocytes l They wondered if CR 3 rearrangement was specific to C. burnetii or was it indicative of any rearrangements of F-actin l Stimulated THP-1 cells with RANTES and was analyzed by transmission electron microscope l Observed pseudopodia similar to that elicited by C. burnetii
cont
cont l Using the same technique they found that beads attached to CD 11 and CD 18 were found in psuedopodal extensions of monocytes stimulated by RANTES(30 and 25% respectively) l The distribution of beads άβ integrin, and IAP were similar to those of C. burnetii This proves that C. burnetii specifically excludes CR 3 from pseudopods
cont
RANTES-mediated restoration of C. burnetii phagocytosis l Treated some cells with RANTES and the other C. burnetii l Then incubated the cells with particles which need CR 3 for optimal binding to monocytes (IC 3 b-coated E, zymosan, and Avirulent C. burnetii)
cont l 40% of particles associated with RANTES treated cells were bound l 20% were associated with C. burnetii treated cells were bound
cont
RANTES effects on C. burnetii treated cells
Nef-mediated restoration on C. Burnetii phagocytosis l They wondered if expression in THP-1 monocytes interferes with C. burnetii phagocytosis as did RANTES stimulation l Transfected Nef into the cells l Introduction of C. burnetii to the Nef transfected cells l Pseudopodal extensions similar to those observed earlier
cont l CD 18 bound beads were present in deformation areas of cells that expressed Nef l The distribution of άβ integrin and IAP were not effected by Nef l The over expression of Nef up regulated the uptake of virulent C. burnetii
cont
CR 3 -depended phagocytosis and src kinases Pretreated THP-1 cells with PP 1, and inhibitor of src kinase l Stimulated the cells with either RANTES or C. l burnetii l l PP 1 did not effect F-actin in RANTES but in C. burnetii cells it significantly inhibited the reorganization of the cells This effect was dose dependent PPI up-regulated C. burnetii uptake by 150% This proves that src is involved in cytoskeleton reorganization C. burnetii induced cells
CR 3 distribution and C. burnetii survival l Since RANTES and Nef expression stimulated Cr 3 redistribution toward pseudopodal extension and increased phagocytosis of C. burnetii l Did this effect the survival l Pretreated cells with RANTES and Nef and then infected with virulent organisms and cultured for 4 days
cont l Then researchers did same experiment but added an anti CR 3 abs l C. burnetii restored its ability to replicate l These results show that the availability of CR 3 impairs C. burnetii replication but does not result in bacteria elimination
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Conclusion l Researchers were able to prove that cytoskeleton reorganization and CR 3 distribution are distinct and controlled by different factors l CR 3 does not kill the bacteria just decreases ability to replicate
My question l Does C. burnetii inhibit CR 3 before or after it gets phagocytosed? Do you have any questions for me?
Well that’s my story and I’m sticking to it
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