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Extraction of Apoplastic Bacteria Using a Syringe-Based Pressure Method

作者：

简介：

Overview

This article describes a method for extracting apoplastic fluid from Arabidopsis and bean plants to study plant-microbe interactions. The process involves creating a closed chamber to apply positive and negative pressure, facilitating the dislodgment of bacteria from plant tissues.

Key Study Components

Area of Science

Plant biology
Microbiology
Plant-microbe interactions

Background

Understanding plant-microbe interactions is crucial for agricultural advancements.
Apoplastic fluid contains important information about microbial colonization.
Arabidopsis and bean plants serve as model organisms in plant research.
Effective extraction methods are necessary for analyzing microbial communities.

Purpose of Study

To develop a reliable method for extracting apoplastic fluid from plant tissues.
To investigate the dynamics of bacterial colonization in plants.
To facilitate further analysis of the extracted fluid for microbial content.

Methods Used

Pre-inoculation of Arabidopsis leaves with bacteria.
Use of a needleless syringe for fluid extraction.
Application of positive and negative pressure to dislodge bacteria.
Collection of apoplastic fluid for subsequent analysis.

Main Results

Successful extraction of apoplastic fluid containing bacteria.
Demonstration of the effectiveness of pressure cycles in dislodging microcolonies.
Establishment of a protocol for studying plant-microbe interactions.
Insights into the behavior of bacteria in the apoplast.

Conclusions

The method provides a valuable tool for researchers studying plant-microbe interactions.
Further studies can utilize the extracted fluid for microbial analysis.
Understanding these interactions can lead to improved agricultural practices.

Frequently Asked Questions

What is apoplastic fluid?

Apoplastic fluid is the liquid found in the intercellular spaces of plant tissues, which can contain various solutes and microorganisms.

Why is studying plant-microbe interactions important?

These interactions can influence plant health, growth, and resistance to diseases, impacting agricultural productivity.

How does the extraction method work?

The method involves creating pressure changes in a syringe to dislodge bacteria from plant tissues without damaging them.

What types of plants were used in this study?

Arabidopsis and bean plants were used as model organisms for the experiments.

What can be analyzed from the extracted apoplastic fluid?

The fluid can be analyzed for microbial content, metabolites, and other biochemical properties relevant to plant-microbe interactions.

Take an Arabidopsis plant with leaves pre-inoculated with bacteria to study plant-microbe interactions.

These bacteria proliferate in the apoplast, the intercellular space between plant cells, forming microcolonies.

Once apoplastic colonization is established, excise the leaves and place them into a needleless syringe.

Add distilled water to cover the tissue.

Insert the plunger, then hold the syringe upright, tap it, and adjust the plunger to release any trapped air.

Seal the tip with parafilm to create a closed chamber for apoplast extraction.

Apply positive pressure by pushing the plunger until the tissue turns dark, indicating compression and water entry into the intercellular spaces to dislodge bacteria.

Next, apply negative pressure by pulling the plunger to expand the tissue matrix and draw out fluid and bacteria.

Repeat the pressure cycles to generate shear forces that disrupt microcolonies, releasing bacteria without damaging the plant tissue.

Unseal the syringe and collect the apoplastic fluid containing dispersed bacteria for further analysis.

Four days after inoculation, cut either the aerial part of the Arabidopsis plant or the inoculated leaf from the bean plant and place it into a 20-milliliter syringe without a needle.

For bean leaves, roll the leaf on itself, leaving the abaxial face outward. Add enough volume of distilled water to cover the tissue. Then, insert the plunger holding the syringe in an upright position and remove the excess air and air bubbles inside the syringe by gently tapping the barrel until all the air is located near the tip, and, after removing the air, cover the tip of the syringe barrel with paraffin film.

Now carefully press the plunger to generate positive pressure until the tissue turns darker. Then, pull the plunger to generate negative pressure. Remove the paraffin film and the plunger and collect the fluid containing the apoplast-extracted bacteria.

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