Table 1.
Advantages and disadvantages of common chemotaxis assays. M- Molar, mM- Millimolar.
Method |
Detection Time |
Molar Concentration |
Advantages |
Disadvantages |
References |
Agar-based assays |
Hard-plug agar assay (HAP assay) |
3 h |
10–100 mM |
-Easy to prepare. -Gives quantitative data. -Requires minimal equipment. -Strains can be compared directly. |
-Chemorepellent taxis are difficult to observe. -False positive results are possible. |
[16] |
Modified hard-plug agar assay (t-HAP assay) |
10 min to 3 h |
10–100 mM |
-Easy to prepare. -Gives quantitative data. -Requires minimal equipment. -Strains can be compared directly. -Differentiations between catabolised and non-catabolised ligands are possible |
-Chemorepellent taxis are difficult to observe. |
[26][27] |
Nutrient-depletion assay |
3–6 h |
2–10 mM |
-Gives quantitative data. -Easy to prepare. -Requires minimal equipment. -Strains can be compared directly. - chemorepellents taxis can be quantitated. -Gradients are created by diffusion, not metabolism. |
-Sensitive to any motions around the assays. -One strain and conditions can be monitored per assay. -Visual observation is difficult. |
[34,35][28][29] |
Tube-based assay |
75 h |
1 M |
-Easy to prepare. -Requires minimal equipment. -Strains can be compared directly. |
-Not suitable for studying chemorepellents. -Semi-quantitative. |
[36][30] |
Capillary assay |
Capillary assay |
1 h |
10–100 mM |
-Gives quantitative data. -Requires minimal equipment. -Gradients are created by diffusion, not metabolism. |
-Not suitable for studying chemorepellents. -One strain and condition can be monitored per assay. |
[37][31] |
Chemotaxis chamber |
μ-slide chemotaxis chamber |
3 h |
5–10 mM |
-Ideal to study the behaviour of a single cell. -Chemoresponses can be measured for a group of cells or a single cell. Clear visualisation of cell migration. -Gives quantitative data. |
-One strain and condition can be monitored per assay. -Tracking system is relatively expensive. |
[38,39][32][33] |
2.2. Tube-Based Chemotaxis Assays
This assay was first described by Reuter et al.
[27][34] for characterisation of the energy taxis genes,
cj1190c (
cetA),
cj1189c (
cetB) and
cj1110c (
cetZ) in
CC. jejuni. jejuni. The assay was adapted by Dwivedi, et al.
[27][34] to investigate the fucose chemotaxis in
CC. jejuni. jejuni. In this Ba
ssay, bacterial cells in 0.4% PBS-agar are transferred to the bottom of a 2 mL Eppendorf tube, allowed to solidify and then overlaid with 1 mL of 0.4% PBS-agar. A filter paper soaked with 50 µL of a chemoeffector (i.e., L-fucose, L-serine) is placed on top of the agar and incubated under microaerobic conditions for 72 h at 37 °C. Bacterial cells that migrate through the upper layer of PBS-agar towards a chemoeffector in the filter paper can be visualised by adding TTC. As TTC changes colour to red in the presence of metabolic activity, the chemoattractant effect can be observed by formation of a red ring of bacterial cells on the top of the tube, visible after 3–4 h of additional incubation
[36,40][30][35]. The additional advantage of this assay is that the bacteria accumulated in the top layer of the agar can be collected and quantitated by viable count allowing the collection of both qualitative and quantitative data. Unfortunately, this assay is not suitable for the assessment of chemorepellents and the 72 h incubation time could lead to an increase in cell number due to growth and can thus affect the measurement of chemotactic activity (
Table 1). The controls
in this assay became even more difficult to design, as different metabolites affect the increase in the bacterial numbers, due to growth, differently.
2.3. Nutrient-Depletion Assay
The nutrient-depletion assay has been developed for the quantitative assessment of both chemoattractants and chemorepellents
[35,41][29][36]. Briefly, 0.5% agar (in H
2O without any nutrients) is poured into a petri dish and plugs of 6 mm are removed and then replaced with 0.5% agar with 2 mM of a chemoeffector. The plates are overlaid with 0.1% agar in H
2O and left for 2 h to allow for the diffusion of chemoeffectors to create a chemical gradient.
C. jejuni cells (~10
8–10
9 cfu/mL) in a 100 μL of bacterial suspension are inoculated in the centre of the petri dish and incubated at 37 °C for 4 h to allow chemotactic migration of the cells. To determine the number of viable bacteria associated with each plug, a 5 mm area around and including each plug is removed and quantitated by viable count. This assay was used to identify ligands for a number of
C. jejuni chemoreceptors.
3. Capillary Assays
The capillary chemotaxis assay had been considered as a “gold standard” for many years and was the most commonly used method to assess bacterial chemotaxis in which errors due to metabolic activity and growth can be minimized
[18,42,43][18][37][38].
In tTh
is assay, the chemotaxis is monitored by measuring the number of bacterial cells entering a capillary tube over a period of hours in the presence or absence of chemoeffectors. In brief, a capillary tube, 1 µL disposable micropipette (3 cm long with an internal diameter of 0.2 mm), containing a solution of an attractant, and sealed at one end, is inserted into a bacterial suspension. A spatial gradient is formed by the diffusion of the attractant/from the tip of the capillary tube. After incubation for 30–60 min, the capillary is removed, and the sealed end is broken off over a test tube containing tryptone broth to be ready for a viable count. For positive chemotaxis, the number of cells accumulated inside a capillary containing attractant solution is measured. For negative chemotaxis, the repellent effector in the capillary decreases the number of cells as opposed to the cell numbers accumulated due to random motion. Driven by the level of handling difficulty, expertise required and low reproducibility, particularly in the assessment of chemorepellents, a number of modifications were introduced over time.
One capillary based assay had been modified to enable the quantitative measurement of bacterial chemoresponses for
Pseudomonas spp.
[44[39][40][41][42],
45,46,47], H. pylori [48][43] and
Campylobacter spp.
[24,37][24][31]. Briefly
, C. jejuni cells are harvested into PBS buffer to OD
600 of 0.5. A 100 μL of a solution containing 100 mM of a chemoeffector is aspirated through a stainless-steel needle (0.25 mm diameter × 20 mm long) into a 1 mL tuberculin syringe. A 100 μL of the bacterial suspension is then drawn into a 200 μL disposable pipette tip, which is then sealed at one end. The needle-syringe system is fitted to a pipette tip in such a way that most of the needle is immersed into the bacterial suspension and incubated horizontally for 1 h allowing the cells to migrate toward an effector. Bacterial cells migrated into the syringe are enumerated by viable count.
4. Slide-Based Chemotaxis Assay
Recently developed microscopic tracking systems can provide a powerful alternative tool to assess bacterial motility and chemotaxis
[52,53,54][44][45][46]. This system allows for a more standardised approach to tracking a group of cells or a single cell through microscopy and time–lapse images measure many features of bacterial motility such as cell migration, velocity, and navigational behavior. A good example is an assay using an agarose-in-plug bridge method, employed to study chemotaxis in many organisms, such as Archaeon
Halobacterium salinarum,
Escherichia coli,
P. putida, and
H. pylori [21,41,55,56,57][21][36][47][48][49]. In principle, two square coverslips are placed on each side of a slide, around 16 mm apart. Agarose plugs are prepared in the middle of the two coverslips by pipetting 5–12 μL of preheated low melting point agarose (LMA), containing the effector to be tested or only PBS as control. Immediately, a third glass coverslip is placed over the bridge, using the edge of the other two coverslips as a stand. The overnight cells are then pipetted between the microscope slide and third glass coverslip and observed by microscopy and photographs are taken of the area at the edges of the plugs after 5–30 min where the chemotactic bands (density of cells) form around the agarose plug. This method is semi-quantitative, aimed at testing attractants and requires skill in assembly of the in-plug bridge. While not used to assess campylobacteria, this method was employed to assess the chemotactic behaviour of
H. salinarum [55][47] and demonstrated the cell migration toward glutamate.
5. Comparison of t-HAP, Nutrient-Depletion and μ-Slide Assays
Nutrient-depletion assay, t-HAP and μ-slide chemotaxis appear to offer the most advantages for assessing both chemoattractant and chemorepellent responses. Here, quantitative data is compared from previously published t-HAP, nutrient-depletion and μ-slide assays
[26,41][27][36] for measurements of the chemotactic motility of
C. jejuni 11168-O, and its
Δtlp10LBD isogenic mutant strain
[39][33]. All three assays were in agreement in establishing the repertoire of chemoattractants and chemorepellents for Tlp10.