O-antigen-deficient francisella tularensis live vaccine strain mutants are ingested via an aberrant form of looping phagocytosis and show altered kinetics of intracellular trafficking in human macrophages

Infection and Immunity
Volume 80, Issue 3, 2012, Pages 952-967

O-antigen-deficient francisella tularensis live vaccine strain mutants are ingested via an aberrant form of looping phagocytosis and show altered kinetics of intracellular trafficking in human macrophages (Article) (Open Access)

Clemens D.L.* , Lee B.-Y. , Horwitz M.A.

^a Division of Infectious Diseases, Department of Medicine, University of California-Los Angeles School of Medicine, Center for Health Sciences, Los Angeles, CA, United States
^b Division of Infectious Diseases, Department of Medicine, University of California-Los Angeles School of Medicine, Center for Health Sciences, Los Angeles, CA, United States
^c Division of Infectious Diseases, Department of Medicine, University of California-Los Angeles School of Medicine, Center for Health Sciences, Los Angeles, CA, United States

Abstract

We examined the uptake and intracellular trafficking of F. tularensis Live Vaccine Strain (LVS) and LVS with disruptions of wbt- DEF and wbtI genes essential for synthesis of the O antigen of lipopolysaccharide. Unlike parental bacteria, O-antigen-deficient LVS is efficiently killed by serum with intact complement but not by serum lacking terminal complement components. Opsonization of O-antigen-deficient LVS in serum lacking terminal complement components allows efficient uptake of these live bacteria by macrophages. In the presence of complement, whereas parental F. tularensis LVS is internalized within spacious pseudopod loops, mutant LVS is internalized within tightly juxtaposed multiple onion-like layers of pseudopodia. Without complement, both parental and mutant LVSs are internalized within spacious pseudopod loops. Thus, molecules other than O antigen are important in triggering dramatic pseudopod extensions and uptake by spacious pseudopod loops. Following uptake, both parental and mutant LVSs enter compartments that show limited staining for the lysosomal membrane glycoprotein CD63 and little fusion with secondary lysosomes. Subsequently, both parental and mutant LVSs lose their CD63 staining. Whereas the majority of parental LVS escapes into the cytosol by 6 h after uptake, mutant LVS shows a marked lag but does escape by 1 day after uptake. Despite the altered kinetics of phagosome escape, both mutant and parental strains grow to high levels within human macrophages. Thus, the O antigen plays a role in the morphology of uptake in the presence of complement and the kinetics of intracellular growth but is not essential for escape, survival, altered membrane trafficking, or intramacrophage growth. © 2012, American Society for Microbiology.

Author Keywords

[No Keywords available]

Index Keywords

Cell Line human controlled study priority journal nonhuman cell migration human cell Humans Article Phagocytosis gene disruption Opsonin Proteins O antigen CD63 antigen Francisella tularensis Phagosomes bacterial cell kinetics lysosome macrophage Bacterial Vaccines O Antigens Complement System Proteins Macrophages Cytosol bacterial survival pseudopodium opsonization Vaccines, Attenuated bacterial strain lipopolysaccharide

Link
https://www.scopus.com/inward/record.uri?eid=2-s2.0-84863275260&doi=10.1128%2fIAI.05221-11&partnerID=40&md5=f17f5f27e35ecc984a7021dcbd5aa64b

DOI: 10.1128/IAI.05221-11

ISSN: 00199567

Cited by: 18

Original Language: English