# Advanced Genetic Tools for Studying Chlamydia

> **NIH NIH R21** · UNIVERSITY OF FLORIDA · 2024 · $188,804

## Abstract

PROJECT SUMMARY/ABSTRACT
Chlamydiae are obligate intracellular bacterial pathogens that cause disease in human and animal populations
Chlamydia trachomatis is the major cause of both bacterial sexually transmitted disease and infectious
blindness in the world. Despite great strides over the past decade, tools for genetic study and manipulation of
Chlamydia spp. remain severely limited. This proposal will develop new and powerful genetic tools including
tightly negatively regulated promoter expression systems, a Tn7-based single chromosomal insertion
transgene system, and application of the latter to build new, smaller shuttle plasmids for transformation.
 Specific Aim 1 – Development of a tightly negatively regulated inducible promoter for Chlamydia.
This aim will provide one of the key missing tools in the repertoire of genetic tools for Chlamydia: a tightly
negatively regulated, inducible, and titratable promoter for performing expression / overexpression studies. In
bacterial physiology studies, it is important to be able to express and overexpress cloned genes in a mutant or
wild type genetic background. One also must be able to tightly repress the cloned gene to avoid undesirable
phenotypes associated with leaky expression of the cloned gene. The two subaims will design and test
inducible promoter systems derived from two well-established Escherichia coli systems: the lac operon and the
arabinose operon. Both systems are tightly repressed in the absence of inducer and rapidly upregulated when
inducer is present. Our rigorous validation plan will use three reporter genes to measure promoter activity
in the presence and absence of inducer. The lac operon promoters will allow us to develop a range of
promoters of varying induction strength and induction ratios to provide flexibility for future genetic studies.
 Specific Aim 2 – Development of a chromosomal Tn7 transgene insertion system for single copy
gene complementation studies in Chlamydia. Shuttle plasmids used in Chlamydia complementation
studies are based on the native Chlamydia plasmid, which is present at 7.6 copies per genome. The major
shortcoming of expressing a cloned gene from a multi-copy plasmid is that even low copies of the plasmid may
lead to non-physiological levels of gene expression and aberrant phenotypes that complicate
interpretation of the complementation results. The Tn7 transgene system provides high frequency, site-
specific, single copy chromosomal insertion of any gene with the additional advantage of removing the
need for antibiotic selection for transgene maintenance. We will adapt the Tn7 transgene system to Chlamydia.
Our proposal includes a rigorous strategy to test the transgene system and plans to optimize the system by
selection for transposase mutants that more efficiently recognize the chlamydial Tn7 attachment site. We
will apply the Tn7 transgene system to build and validate new, smaller shuttle plasmids, which should
improve transformation efficiencie...

## Key facts

- **NIH application ID:** 10911787
- **Project number:** 5R21AI169341-02
- **Recipient organization:** UNIVERSITY OF FLORIDA
- **Principal Investigator:** Anthony T Maurelli
- **Activity code:** R21 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2024
- **Award amount:** $188,804
- **Award type:** 5
- **Project period:** 2023-08-22 → 2026-01-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10911787

## Citation

> US National Institutes of Health, RePORTER application 10911787, Advanced Genetic Tools for Studying Chlamydia (5R21AI169341-02). Retrieved via AI Analytics 2026-05-25 from https://api.ai-analytics.org/grant/nih/10911787. Licensed CC0.

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