# Rickettsia conorii transposon mutagenesis and spotted fever pathogenesis

> **NIH NIH R21** · STATE UNIVERSITY NEW YORK STONY BROOK · 2020 · $199,375

## Abstract

ABSTRACT
Rickettsia are obligate intracellular bacteria of the a-proteobacteria family impacting human development as
causative agents of Typhus and Spotted Fever. Hallmark of Rickettsia is their replication in human vascular
endothelial cells, release into the bloodstream and transmission via hematophagic arthropods, with Rickettsia
replicating in the gastrointestinal tract or salivary glands of various vectors (lice, ticks, mites or fleas). Owing to
technical difficulties of isolating and propagating Rickettsia, Typhus and Spotted Fever have long been
diagnosed via serological agglutination for antibodies cross-reactive with Proteus vulgaris (Weil-Felix reaction).
For epidemic Typhus, positive Weil-Felix serology is associated with survival and with the development of
immunity that, if waning, may precipitate recrudescent typhus with recall of Weil-Felix serology. Early work
developed vaccines successful at preventing epidemic Typhus, however the mechanisms for protective
immunity are still unknown. To explore the genetic bases of rickettsial pathogenesis, several laboratories
developed technologies for generating mutations in Rickettsia. This work identified mutants with defects in
actin-based motility and cell-to-cell spread. Nevertheless, genes underpinning rickettsial entry into vascular
endothelial cells, intracellular replication, release into the bloodstream or replication in various cell types of
their insect vectors remain largely unknown. Here we describe an in vitro transposition reaction using purified
Tn5-transposase complexed with mini-transposon, which provides for chloramphenicol-selection of Rickettsia
conorii variants with chromosomal insertions. DNA sequencing of insertion sites demonstrates the random
nature of insertional mutagenesis with the mini-transposon, while chloramphenicol-selection allows for facile
isolation of variants that can be analyzed for in vitro replication as well as defects in the pathogenesis of
Boutonneuse Fever. One of the isolated R. conorii variants, with insertion in the polysaccharide synthesis
operon (pso), exhibits defects in attachment and invasion of tissue culture cells and in Spotted Fever
pathogenesis in mice. The disrupted gene encodes an enzyme predicted to synthesize QuiNAc, a structural
determinant in the lipopolysaccharide of P. vulgaris OX19. As the pso locus encompasses genes that are
conserved or variable among different rickettsial species, these data suggest that lipopolysaccharide of R.
conorii contributes to the Rickettsia replicative life-style, elicits immune responses that define serological cross-
reactivity with P. vulgaris (Weil-Felix serology) and may represent a determinant of antibody-mediated
immunity. To further the genetic analysis of Rickettsia, we propose to use insertional mutagenesis to generate
a library of R. conorii transposon mutants. These mutants will be screened for replication defects in human
vascular endothelial cells and phenotypic variants will be cha...

## Key facts

- **NIH application ID:** 10071364
- **Project number:** 7R21AI144136-02
- **Recipient organization:** STATE UNIVERSITY NEW YORK STONY BROOK
- **Principal Investigator:** Hwan Keun Kim
- **Activity code:** R21 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $199,375
- **Award type:** 7
- **Project period:** 2020-01-01 → 2021-12-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10071364

## Citation

> US National Institutes of Health, RePORTER application 10071364, Rickettsia conorii transposon mutagenesis and spotted fever pathogenesis (7R21AI144136-02). Retrieved via AI Analytics 2026-05-21 from https://api.ai-analytics.org/grant/nih/10071364. Licensed CC0.

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