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Modeling Aeromonas Pathogenesis in C. elegans Using a Survival Assay

作者：

简介：

Overview

This study investigates the pathogenic effects of Aeromonas strains on C. elegans, a model organism. The experiment assesses bacterial colonization and its impact on nematode survival.

Key Study Components

Area of Science

Microbiology
Pathogenesis
Model Organisms

Background

Aeromonas is a bacterial pathogen known to affect various hosts.
C. elegans serves as a valuable model for studying host-pathogen interactions.
Understanding bacterial effects on nematodes can provide insights into pathogenic mechanisms.
Survival analysis is crucial for evaluating host viability in response to infection.

Purpose of Study

To examine the effects of Aeromonas strains on the survival of C. elegans.
To assess the bacterial colonization process within the nematode.
To generate survival curves to quantify host mortality over time.

Methods Used

Culturing Aeromonas strains in nutrient-rich media.
Measuring optical density to standardize bacterial concentration.
Inoculating C. elegans larvae onto bacterial layers for infection.
Daily monitoring and counting of live and dead nematodes.

Main Results

Bacteria multiply within the nematode, leading to intestinal damage.
Survival curves indicate the mortality rate of C. elegans over time.
Different Aeromonas strains exhibit varying pathogenic effects.
Daily counts provide insights into the dynamics of host response.

Conclusions

Aeromonas strains significantly impact the survival of C. elegans.
The study highlights the utility of C. elegans in pathogenicity research.
Findings contribute to understanding host-pathogen interactions.

Frequently Asked Questions

What is the significance of using C. elegans in this study?

C. elegans is a well-established model organism that allows researchers to study host-pathogen interactions in a controlled environment.

How are the survival curves generated?

Survival curves are created by counting the number of live, dead, and unresponsive nematodes daily until all worms have died.

What are the implications of this research?

The findings can help in understanding the mechanisms of bacterial pathogenesis and the host's immune response.

How does Aeromonas affect C. elegans?

Aeromonas multiplies in the nematode's intestine, releasing cytotoxins that damage epithelial cells and lead to mortality.

What methods are used to culture Aeromonas?

Aeromonas strains are cultured in nutrient-rich media, and their concentration is adjusted based on optical density measurements.

What temperature is used for incubating the plates?

The plates are incubated at 20 degrees Celsius to facilitate bacterial growth and nematode infection.

Begin with a culture of an Aeromonas strain, a bacterial pathogen, grown in a nutrient-rich medium.

Measure the optical density of the culture and adjust the bacterial concentration to ensure a consistent infection load.

Plate the culture onto nematode growth medium or NGM agar and incubate to form a uniform bacterial layer.

Prepare developmentally synchronized C. elegans larvae-a bacterivorous nematode maintained on an enriched medium.

Transfer the larvae onto the bacterial layer and incubate to allow oral ingestion of Aeromonas and enable intestinal colonization.

Inside the host, the bacteria multiply and release cytotoxins that damage intestinal epithelial cells, and lead to mortality.

Transfer surviving nematodes onto fresh bacterial plates and count the number of live, dead, and unresponsive worms daily until the last worm dies.

Finally, generate a survival curve to assess host viability over time.

First, select a single colony of each of the four Aeromonas strains and culture them according to the text protocol. Then, measure the OD₆₀₀ absorbance of the bacterial broth and adjust it until the absorbance is equal to 2.0.

Next spot and spread 30 microliters of bacterial broth from each strain into NGM plates.

Randomly select and transfer the previously prepared L4 worms to the NGM plates with the Aeromonas strains. Then, incubate the plates at 20 degrees Celsius until the assay is complete.

Every day transfer all of the living worms to a new NGM plate with bacteria. Count the numbers of living, dead, and sensor worms every day until the last worm is dead.

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