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Biologia

Визуализация Бактерии в Нематоды использованием флуоресцентной микроскопии

Published: October 19, 2012
doi:
10.3791/4298
, ,
1Department of Bacteriology,University of Wisconsin-Madison

Summary

Для изучения взаимности между<em> Xenorhabdus</em> Бактерий и<em> Steinernema</em> Нематод, были разработаны методы для контроля бактериальной наличие и расположение в пределах нематод. Экспериментальный подход, который может быть применен к другим системам, влечет за собой инженерные бактерии, чтобы выразить зеленый флуоресцентный белок и визуализации, с помощью флуоресцентной микроскопии бактерий в прозрачном нематоды.

Abstract

Symbioses, the living together of two or more organisms, are widespread throughout all kingdoms of life. As two of the most ubiquitous organisms on earth, nematodes and bacteria form a wide array of symbiotic associations that range from beneficial to pathogenic 1-3. One such association is the mutually beneficial relationship between Xenorhabdus bacteria and Steinernema nematodes, which has emerged as a model system of symbiosis 4. Steinernema nematodes are entomopathogenic, using their bacterial symbiont to kill insects 5. For transmission between insect hosts, the bacteria colonize the intestine of the nematode’s infective juvenile stage 6-8. Recently, several other nematode species have been shown to utilize bacteria to kill insects 9-13, and investigations have begun examining the interactions between the nematodes and bacteria in these systems 9.

We describe a method for visualization of a bacterial symbiont within or on a nematode host, taking advantage of the optical transparency of nematodes when viewed by microscopy. The bacteria are engineered to express a fluorescent protein, allowing their visualization by fluorescence microscopy. Many plasmids are available that carry genes encoding proteins that fluoresce at different wavelengths (i.e. green or red), and conjugation of plasmids from a donor Escherichia coli strain into a recipient bacterial symbiont is successful for a broad range of bacteria. The methods described were developed to investigate the association between Steinernema carpocapsae and Xenorhabdus nematophila 14. Similar methods have been used to investigate other nematode-bacterium associations 9,15-18and the approach therefore is generally applicable.

The method allows characterization of bacterial presence and localization within nematodes at different stages of development, providing insights into the nature of the association and the process of colonization 14,16,19. Microscopic analysis reveals both colonization frequency within a population and localization of bacteria to host tissues 14,16,19-21. This is an advantage over other methods of monitoring bacteria within nematode populations, such as sonication 22or grinding 23, which can provide average levels of colonization, but may not, for example, discriminate populations with a high frequency of low symbiont loads from populations with a low frequency of high symbiont loads. Discriminating the frequency and load of colonizing bacteria can be especially important when screening or characterizing bacterial mutants for colonization phenotypes 21,24. Indeed, fluorescence microscopy has been used in high throughput screening of bacterial mutants for defects in colonization 17,18, and is less laborious than other methods, including sonication 22,25-27and individual nematode dissection 28,29.

Protocol

1. Строительство Флуоресцентные бактериальный штамм с помощью сопряжения Расти получателя деформации (симбионт должны быть рассмотрены) и доноров штамм в течение ночи. Донор деформации, как правило, кишечная палочка, должны быть способны отдавать ДНК через сопряжение и долж…

Discussion

Протокол, описанный здесь, предоставляет метод для оптического обнаружения бактерий в нематодой хост (рис. 1). Этот метод использует оптическую прозрачность нематод и способности флуоресцентной меткой бактерий, что позволяет в естественных условиях анализа бактерий в не…

Divulgazioni

The authors have nothing to disclose.

Acknowledgements

Авторы хотели бы поблагодарить Eugenio Vivas, Курт Heungens, Эрик Мартенс, Чарльз Cowles, Дарби Sugar, Eric Стабб, и Тодд Ciche за их вклад в развитие этого протокола и инструменты, используемые. KEM и СКМ при поддержке Национального института здоровья (NIH) Национального исследовательского Service Award T32 (AI55397 "микробы в норме и патологии»). СКМ при поддержке Национального научного фонда (NSF) Высшее Research Fellowship. Эта работа была поддержана грантами от Национального научного фонда (IOS-0920631 и IOS-0950873).

Materials

Name of the reagent Company Catalogue number Comments (optional)
Lipid Agar
(sterile)		 8 grams nutrient broth, 15 grams agar, 5 grams yeast extract, 890 ml water, 10 ml 0.2 g/ml MgCl2. 6H20, 96 ml corn syrup solution*, 4 ml corn oil*
Stir media while pouring plates
*add sterile ingredient after autoclaving
Corn Syrup Solution
(sterile)		 7 ml corn syrup, 89 ml water
mix and autoclave
Egg Solution 16.6 ml 12% sodium hypochlorite, 5 ml 5M KOH, 80 ml water
Lysogeny Broth
(sterile)		 5 grams yeast extract, 10 grams tryptone, 5 grams salt, 1 L water
mix and autoclave
Microfuge Fisher 13-100-675 Any microfuge that holds microfuge tubes will work
Centrifuge Beckman 366802 Large table top centrifuge that holds 15 ml and 50 ml conical tubes
Sterile 60 mm X 15 mm Petri Dish Fisher 0875713
50 ml centrifuge tubes Fisher 05-539-6
15 ml centrifuge tubes Fisher 05-531-6
Sterile 100 mm X 20 mm Petri Dish Fisher 0875711Z Deeper than standard Petri dishes
24-well plate Greiner Bio-One 662000-06
Microscope The microscope needs florescent capabilities compatible with your fluorophore
Paraformaldehyde Electron Microscopy Sciences 15710
PBS
(sterile)		 8 g NaCL
0.2 g KCL
1.44 g Na2HPO4
0.24 g KH2PO4
1 L water

Adjust to a pH of 7.4 and water to 1 L and autoclave
Microfuge tubes Fisher 05-408-138 2 ml or 1.5 ml tubes
Shaker Any shaker that causes the liquid to gently move will work
Diaminopimelic acid Sigma D-1377 If needed, supplement media to a concentration or 1 mM
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Riferimenti

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Tags

VisualizingBacteriaNematodesFluorescent MicroscopySymbiotic AssociationsXenorhabdus BacteriaSteinernema NematodesModel SystemEntomopathogenicBacterial SymbiontIntestineInfective Juvenile StageNematode SpeciesInteractionsVisualization MethodOptical TransparencyMicroscopyFluorescent ProteinPlasmidsEscherichia Coli Strain
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Murfin, K. E., Chaston, J., Goodrich-Blair, H. Visualizing Bacteria in Nematodes using Fluorescent Microscopy. J. Vis. Exp. (68), e4298, doi:10.3791/4298 (2012).
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