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W tym Artykule

  • Podsumowanie
  • Streszczenie
  • Wprowadzenie
  • Protokół
  • Wyniki
  • Dyskusje
  • Ujawnienia
  • Podziękowania
  • Materiały
  • Odniesienia
  • Przedruki i uprawnienia

Podsumowanie

A technique to study NG2 cells and oligodendrocytes using a slice culture system of the forebrain and cerebellum is described. This method allows examination of the dynamics of proliferation and differentiation of cells within the oligodendrocyte lineage where the extracellular environment can be easily manipulated while maintaining tissue cytoarchitecture.

Streszczenie

NG2 expressing cells (polydendrocytes, oligodendrocyte precursor cells) are the fourth major glial cell population in the central nervous system. During embryonic and postnatal development they actively proliferate and generate myelinating oligodendrocytes. These cells have commonly been studied in primary dissociated cultures, neuron cocultures, and in fixed tissue. Using newly available transgenic mouse lines slice culture systems can be used to investigate proliferation and differentiation of oligodendrocyte lineage cells in both gray and white matter regions of the forebrain and cerebellum. Slice cultures are prepared from early postnatal mice and are kept in culture for up to 1 month. These slices can be imaged multiple times over the culture period to investigate cellular behavior and interactions. This method allows visualization of NG2 cell division and the steps leading to oligodendrocyte differentiation while enabling detailed analysis of region-dependent NG2 cell and oligodendrocyte functional heterogeneity. This is a powerful technique that can be used to investigate the intrinsic and extrinsic signals influencing these cells over time in a cellular environment that closely resembles that found in vivo.

Wprowadzenie

Organoytpic slice cultures of the central nervous system have proven to be extremely useful for studying neuron and glial cell biology in a semiintact system14. These cultures are relatively simple to adopt and retain many benefits of primary dissociated cell cultures such as manipulation of the extracellular environment and easy access for repeated long-term live cell imaging and electrophysiological recordings59. In addition, slice cultures maintain 3-dimensional tissue cytoarchitecture, regional neural connectivity, and most major cell types are present in the system. These properties make these cultures a unique and convenient system to investigate single cell behavior and physiology with cellular and environmental interactions.

NG2 cells are a population of glial cells in the mammalian central nervous system that continue to proliferate and generate myelinating oligodendrocytes during embryonic and postnatal development10. They have been extensively studied in dissociated primary cell cultures, and recent development of transgenic mouse lines with NG2 cell-specific expression of fluorescent proteins has facilitated in vivo fate mapping and electrophysiological recordings in acute slice preparations. Even with these studies, little is known about the temporal dynamics of NG2 cell proliferation and oligodendrocyte differentiation. Although dissociated cell culture is widely used for the relative facility in pharmacological and genetic manipulations, it is not suitable for interrogating functional differences of these cells in different brain regions particularly when it is desirable to maintain the context of the cellular microenvironment. Slice cultures provide a simple alternative that is amenable to pharmacological manipulations and have been used to investigate oligodendrocyte myelination11,12, cellular response after lysolecithin (LPC) or antibody induced demyelination13,14, and induction of remyelination via pharmacological treatment15.

A method to investigate and perform live imaging and fixed tissue (or postfixation) analysis of NG2 cell proliferation and oligodendrocyte differentiation in organotypic slice cultures taken from both the forebrain and cerebellum is described. This is a powerful method that can be used to study the cell fate of single NG2 cells after division16 and to discover region- and age-dependent differences in growth factor induced NG2 cell proliferation17. This relatively simple technique is widely accessible to further investigate cell intrinsic and/or environmental mechanisms regulating the physiology of these glial cells and their response to neuronal activity or myelin damage.

Protokół

NOTE: All animal procedures are following the guidelines and have been approved by the Institutional Animal Care and Use Committee (IACUC) at the University of Connecticut.

NOTE: For these experiments constitutive NG2cre18 (JAX#008533) and inducible NG2creER16 (JAX#008538) transgenic mice crossed to Z/EG19 (JAX#003920) or gtRosa26:YFP reporter20 (JAX#006148) lines respectively were used to image NG2 cells and their progeny. To image mature oligodendrocytes, PLPDsRed transgenic mice21 were used. For consistent survival, slices can be isolated from mice up to postnatal day 10 from both the forebrain and cerebellum.

1. Slice Preparation

  1. In a culture hood, place tissue culture inserts in six well plates and add 1 ml slice culture medium (recipe in reagents section). Put the plates in the cell culture incubator at 37 °C with 5% CO2 at least 2 hr prior to dissection.
  2. Sterilize all tools and tissue chopper with 70% ethanol.
  3. Bubble dissection buffer (recipe in reagents section) with 95%  O2, 5% CO2 on ice for at least 15 min prior to the start of dissection.
  4. Anesthetize mouse pups by placing them on ice for 5-10 min according to approved animal protocols. Ascertain the appropriate depth of anesthesia by confirming that the mice do not respond to tail and toe pinching.
  5. Decapitate animals using sharp scissors following animal protocols. Quickly remove the skull over the forebrain and cerebellum by first making a sagittal cut followed by lateral incision, using sterilized tools. Cut cranial nerves from the ventral surface of the brain and cerebellum by carefully rolling the tissue to the side.
  6. Place tissue in a sterile 35 mm dish containing ice-cold oxygenated dissection buffer.
  7. Using a razor blade, sever the cerebellum and forebrain. Then make a mid-sagittal cut through the forebrain and cerebellum, separating the hemispheres.
  8. Cut 300 μm-thick coronal and sagittal sections of the forebrain and cerebellum with a manual tissue chopper. NOTE: A manual tissue chopper allows rapid processing from dissection to culture incubation without the need for agarose embedding. A vibratome can also be used as described previously9.
  9. Transfer separated slices into freshly bubbled cold dissection buffer on ice.
  10. Use small dissecting or weighing spatulas to separate individual sections and transfer them to preincubated six well dishes with culture inserts.
  11. Remove any excess dissection buffer from the surface of the culture insert using a disposable transfer pipette or a P 200 pipet tip. Two to three forebrain or three cerebellar slices can be placed on one culture insert.
    NOTE: For consistent results with forebrain cultures, it is ideal to take slices spanning the anterior one-third of the corpus callosum (Figure 1A) in order to study both gray and white matter regions in the same slice. Each animal usually yields 6 forebrain slices and 6 cerebellum slices.
  12. Place the six well plates in the incubator and replace the slice medium with 1 ml of slice medium 1 day after slice preparation and then every other day until slice fixation.
  13. Depending on the experiment, use slices after 5-7 days in culture. Use only slices that become transparent after the first few days and discard those that have uneven opaque regions. NOTE: Opaque regions within slices are visible by eye and appear as a clump of dark cells under phase contrast. After the technique has been mastered, dead opaque slices occur rarely, in less than 1-5% of slices.

2. Time-Lapse Imaging of NG2 cell Division and Oligodendrocyte Differentiation

NOTE: To perform time lapse imaging of NG2 cell proliferation and differentiation we use NG2cre:ZEG mice16 which express EGFP in NG2 cells and their progeny (Figure 1C-E). Reporter expression in this line is sufficiently robust to obtain live images of GFP+ cells in slices immediately after sectioning for a time period of at least four weeks. The clearest images are obtained after the initial thinning period of the slice, which occurs over the first 3-5 days in culture.

  1. Throughout the experiment, keep the slices in a cell culture incubator at 37 °C and remove only for brief periods of time (less than 15 min per slice), keeping the lid on the six well plate while imaging.
  2. Using an inverted fluorescence microscope equipped with a digital camera, capture images at the first time point using a 10X objective. NOTE: First time points will vary by experiment and can be the day when the slices were prepared or any time point after.
  3. Capture images from multiple regions at time point one in both gray and white matter areas of the slice. Note the region imaged by specific landmarks within the slice and by mapping the image location on a schematic that can be used for subsequent imaging sessions. Useful landmarks can include edges of the slices and/or orientation of white matter tracts. Image four to eight locations on each slice at each time point.
  4. Capture subsequent images at an interval of 4-6 hr if examining NG2 cell division and oligodendrocyte differentiation, ideally over 5-7 days.
  5. Capture a final image of all regions and fix the slices immediately. Add 1 ml of fixative (4% PFA with 0.1M l-lysine 0.01 M sodium meta-periodate) to the bottom of the culture insert, then add another 1 ml on top of the slices. Take care not to squirt the fixative directly on the slice as it can detach from the membrane. Fix the tissue for 30 min  and proceed with immunohistochemistry using developmental stage-specific markers as described in section 4.
  6. Wash slices with 0.2 M sodium phosphate buffer 3 x 10 min. If necessary, store slices at 4 °C in 0.2 M sodium phosphate buffer for 1-3 days before immunostaining but ideally perform staining within 24 hr. Proceed with immunohistochemistry as described below in section 4 to determine the proportion of cells that have differentiated into oligodendrocytes (Figure 2D-F).

3. Fate Mapping of NG2 cell Progeny Using Inducible Reporter Transgenic Mice in Slice Cultures

NOTE: To track the fate of NG2 cells from a particular time point in the culture, inducible NG2creER:YFP transgenic mice can be used.

  1. Induce Cre recombination and reporter expression by adding 100 nM 4OHT dissolved in ethanol to the culture medium. NOTE: Reporter positive cells should appear within 1-2 days at an induction efficiency of ~20-25% YFP+NG2+/NG2+ cells and at this time point will all be cells at the NG2 cell stage (Figure 2A-C)
  2. Fix and wash the slices at different time points after various manipulations (described in sections 2.5 and 2.6).

4. Slice Immunohistochemistry

  1. Cut the membranes with the slices attached out of the inserts using a scalpel.
  2. Transfer slices to individual wells of a 24 well plate containing phosphate buffered saline (PBS) using a set of tweezers, taking care not to disrupt the composition of the slice when picking up the membrane.
  3. Transfer the slices to a 24 well plate with blocking solution containing 5% normal goat serum (NGS) and 0.1% Triton-X100 in PBS for 1 hr.
  4. Incubate the slices in primary antibody O/N in 5% NGS in PBS at 4 °C. For identifying cells in the NG2 cell stage, use antibodies to NG2 and PDGFRα. For identifying differentiated oligodendrocytes, use an antibody to the adenomatous polyposis coli antigen (APC; clone CC1).
  5. On the second day wash slices in PBS 3 x15 min, then incubate in secondary antibodies in 5% NGS in PBS for 1 hr at RT. Wash slices in PBS 3 x15 min and mount on slides. Mount with slices up and membrane facing the slide so that the membrane will not be between the objective and the tissue.

Wyniki

Examples of representative data are given below that have been obtained using slice cultures from both the forebrain and cerebellum of P8 NG2cre:ZEG, NG2creER:YFP and PLPDsRed transgenic mouse lines. NG2 cells can be imaged over days in forebrain and cerebellum slices (Figure 1B-D, Video 1) and the phenotype of these cells can be determined after fixation and immunostaining with NG2 and CC1 antibodies (Figure 1E). In addition to live imaging, cell proliferation can also be assessed using...

Dyskusje

Myelination in the central nervous system is essential for efficient neuronal communication and axonal survival22. NG2 cells continuously generate myelinating oligodendrocytes into adulthood while maintaining a resident population in most brain regions16,2325. Some genetic and molecular mechanisms regulating the differentiation of these cells have been described but much remains to be discovered. Organotypic slice cultures are a convenient tool to investigate these mecha...

Ujawnienia

The authors declare that they have no competing financial interests

Podziękowania

This work was funded by grants from the National Multiple Sclerosis Society (RG4179 to A.N.), the National Institutes of Health (NIH R01NS073425 and R01NS074870 to A.N.) and the National Science Foundation (A.N.). We thank Dr. Frank Kirchhoff (University of Saarland, Homburg Germany) for providing PLPDsRed transgenic mice. We thank Youfen Sun for her assistance in maintaining the transgenic mouse colony.

Materiały

NameCompanyCatalog NumberComments
Slice Culture Medium
Minimum Essential MediumInvitrogen1109050%
Hank’s Balanced Salt SolutionInvitrogen1417525%
HEPESSigma-AldrichH-403425mM
L-GlutamineInvitrogen250301mM
InsulinSigma-AldrichI66341mg/L
Ascorbic AcidSigma-AldrichA-02780.4mM
Horse SerumHycloneSH30074.0325%
Titrate to pH 7.22 with NaOH, filter with bottle top filter, and store at 4 degrees Celsius
Dissection Buffer
NaClSigma-AldrichS3014124mM
KClSigma-AldrichP54053.004mM
KH2PO4Sigma-AldrichP56551.25mM
MgSO4 (anhydrous)Sigma-AldrichM75064.004mM
CaCl2 2H2OSigma-AldrichC79022mM
NaHCO3Sigma-AldrichS576126mM
D-(+)-GlucoseSigma-AldrichG702110mM
Ascorbic AcidSigma-AldrichA-02782.0mM
AdenosineSigma-AldrichA40360.075mM
Filter with bottle top filter and store at 4 degrees Celsius, oxygenate with 95%O2 5%CO2 before use
Other Reagents and Supplies
4-hydroxy tamoxifen (4OHT)Sigma-AldrichH7904100nM
Paraformaldehyde (PFA)EM Sciences192004%
L-LysineSigma-AldrichL-60270.1M
Sodium MetaperiodateSigma-AldrichS-18780.01M
Rabbit anti NG2 antibodyChemicon (Millipore)AB53201:500
Mouse anti CC1 antibodyCalbiochem (Millipore)OP801:200
Mouse anti Ki67 antibodyVision BiosystemsNCL-Ki67-MM11:300
Mouse anti NeuN antibodyChemicon (Millipore)MAB3771:500
Species specific secondary antibodiesJackson Immunoresearch
Normal Goat Serum (NGS)5%
Triton X-1000.10%
Mounting medium with DAPIVector LabsH-1200
Millicell culture membrane inserts 0.45μm pore sizeFisher ScientificPICM03050
Bottle top filtersFisher Scientific09-740-25E
Ethanol
95% O2 5% CO2 gas mix
Phosphate Buffered Saline (PBS)
Sterile six well plates
Dissecting (hippocampal) or weighing spatulas
Manual or automatic tissue chopper
Razor blades
Disposable transfer pipettes
35mm and 60mm sterile Petri dishes
Stereomicroscope
Inverted Phase Microscope
Laminar Flow Hood
Tissue Culture Incubator
Inverted Fluorescence Microcope

Odniesienia

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Keywords Organotypic Slice CulturesOligodendrocyte DynamicsMyelinationNG2 CellsPolydendrocytesOligodendrocyte Precursor CellsPrimary Dissociated CulturesNeuron CoculturesTransgenic Mouse LinesForebrainCerebellumCellular BehaviorCellular InteractionsRegion dependent Heterogeneity

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