Anterograde tracing

In neuroscience, anterograde tracing is a research method which is used to trace axonal projections from their source (the cell body or soma) to their point of termination (the synapse). The complementary technique is retrograde tracing, which is used to trace neural connections from their termination to their source (i.e. synapse to cell body).[1] Both the anterograde and retrograde tracing techniques are based on the visualization of the biological process of axonal transport.

The anterograde and retrograde tracing techniques allow the detailed descriptions of neuronal projections from a single neuron or a defined population of neurons to their various targets throughout the nervous system. These techniques allow the "mapping" of connections between neurons in a particular structure (e.g. the eye) and the target neurons in the brain. Much of what is currently known about connectional neuroanatomy was discovered through the use of the anterograde and retrograde tracing techniques.[1]

Techniques

Several methods exist to trace projections originating from the soma towards their target areas. These techniques initially relied upon the direct physical injection of various visualizable tracer molecules (e.g. Green fluorescent protein, lipophylic dyes or radioactively tagged amino acids) into the brain. These molecules are absorbed locally by the soma (cell body) of various neurons and transported to the axon terminals, or they are absorbed by axons and transported to the soma of the neuron. Other tracer molecules allow for the visualization of large networks of axonal projections extending from the neurons exposed to the tracer.[1]

Over the recent years viral vectors have been developed and implemented as anterograde tracers to identify the target regions of projecting neurons.[2][3]

Alternatively strategies are transsynaptic anterograde tracers, which can cross the synaptic cleft, labeling multiple neurons within a pathway. Those can also be genetic or molecular tracers.

Genetic tracers

(see also Viral neuronal tracing)

In order to trace projections from a specific region or cell, a genetic construct, virus or protein can be locally injected, after which it is allowed to be transported anterogradely. Viral tracers can cross the synapse, and can be used to trace connectivity between brain regions across many synapses. Examples of viruses used for anterograde tracing are described by Kuypers.[4] Most well known are the Herpes simplex virus type1 (HSV) and the Rhabdoviruses.[4] HSV was used to trace the connections between the brain and the stomach, in order to examine the brain areas involved in viscero-sensory processing.[5] Another study used HSV type1 and type2 to investigate the optical pathway: by injecting the virus into the eye, the pathway from the retina into the brain was visualized.[6]

Viral tracers use a receptor on the host cell to attach to it and are then endocytosed. For example, HSV uses the nectin receptor and is then endocytosed. After endocytosis, the low pH inside the vesicle strips the envelope of the virion after which the virus is ready to be transported to the cell body. It was shown that pH and endocytosis are crucial for the HSV to infect a cell.[7] Transport of the viral particles along the axon was shown to depend on the microtubular cytoskeleton.[8]

Molecular tracers

There is also a group of tracers that consist of protein products that can be taken up by the cell and transported across the synapse into the next cell. Wheat-germ agglutinin (WGA) and Phaseolus vulgaris leucoagglutinin[9] are the most well known tracers, however they are not strict anterograde tracers: especially WGA is known to be transported anterogradely as well as retrogradely.[10] WGA enters the cell by binding to Oligosaccharides,and is then taken up via endocytosis via a caveolae-dependent pathway.[11][12]

Other anterograde tracers widely used in neuroanatomy are the biotinylated dextran amines (BDA), also used in retrograde labeling.

Partial list of studies using this technique

The anterograde tracing technique is now a widespread research technique. The following are a partial list of studies that have used anterograde tracing techniques:

See also

References

  1. 1 2 3 Dale Purves; George J. Augustine; David Fitzpatrick; William C. Hall; Anthony-Samuel Lamantia; James O. Mcnamara; Leonard E. White, eds. (2008). Neuroscience (4th ed.). Sunderland, Massachusetts: Sinauer. pp. 16–18 (of 857 total). ISBN 978-0-87893-697-7.
  2. Oh SW; Harris JA; Ng L; et al. (Apr 2014). "A mesoscale connectome of the mouse brain". Nature. 508 (7495): 207–14. doi:10.1038/nature13186. PMID 24695228.
  3. Haberl MG, Viana da Silva S, Guest JM, Ginger M, Ghanem A, Mulle C, Oberlaender M, Conzelmann KK, Frick A (Apr 2014). "An anterograde rabies virus vector for high-resolution large-scale reconstruction of 3D neuron morphology.". Brain Struct Funct. doi:10.1007/s00429-014-0730-z. PMID 24723034.
  4. 1 2 Kuypers HG, Ugolini G (February 1990). "Viruses as transneuronal tracers". Trends in Neurosciences. 13 (2): 71–5. doi:10.1016/0166-2236(90)90071-H. PMID 1690933.
  5. Rinaman L, Schwartz G (March 2004). "Anterograde transneuronal viral tracing of central viscerosensory pathways in rats". The Journal of Neuroscience. 24 (11): 2782–6. doi:10.1523/JNEUROSCI.5329-03.2004. PMID 15028771.
  6. Norgren RB, McLean JH, Bubel HC, Wander A, Bernstein DI, Lehman MN (March 1992). "Anterograde transport of HSV-1 and HSV-2 in the visual system". Brain Research Bulletin. 28 (3): 393–9. doi:10.1016/0361-9230(92)90038-Y. PMID 1317240.
  7. Nicola AV, McEvoy AM, Straus SE (May 2003). "Roles for Endocytosis and Low pH in Herpes Simplex Virus Entry into HeLa and Chinese Hamster Ovary Cells". Journal of Virology. 77 (9): 5324–32. doi:10.1128/JVI.77.9.5324-5332.2003. PMC 153978Freely accessible. PMID 12692234.
  8. Kristensson K, Lycke E, Röyttä M, Svennerholm B, Vahlne A (September 1986). "Neuritic transport of herpes simplex virus in rat sensory neurons in vitro. Effects of substances interacting with microtubular function and axonal flow [nocodazole, taxol and erythro-9-3-(2-hydroxynonyl)adenine]". The Journal of General Virology. 67 (9): 2023–8. doi:10.1099/0022-1317-67-9-2023. PMID 2427647.
  9. Smith Y, Hazrati LN, Parent A (April 1990). "Efferent projections of the subthalamic nucleus in the squirrel monkey as studied by the PHA-L anterograde tracing method". The Journal of Comparative Neurology. 294 (2): 306–23. doi:10.1002/cne.902940213. PMID 2332533.
  10. Damak S, Mosinger B, Margolskee RF (2008). "Transsynaptic transport of wheat germ agglutinin expressed in a subset of type II taste cells of transgenic mice". BMC Neuroscience. 9: 96. doi:10.1186/1471-2202-9-96. PMC 2571104Freely accessible. PMID 18831764.
  11. Broadwell RD, Balin BJ (December 1985). "Endocytic and exocytic pathways of the neuronal secretory process and trans-synaptic transfer of wheat germ agglutinin-horseradish peroxidase in vivo". The Journal of Comparative Neurology. 242 (4): 632–50. doi:10.1002/cne.902420410. PMID 2418083.
  12. Gao X, Wang T, Wu B, et al. (December 2008). "Quantum dots for tracking cellular transport of lectin-functionalized nanoparticles". Biochemical and Biophysical Research Communications. 377 (1): 35–40. doi:10.1016/j.bbrc.2008.09.077. PMID 18823949.
This article is issued from Wikipedia - version of the 5/18/2016. The text is available under the Creative Commons Attribution/Share Alike but additional terms may apply for the media files.