Whole brain mapping of inputs
to inhibitory interneurons
in prefrontal cortex
Yang Xuan
Carlén Lab
Networks for Networks
28th Nov 2014
yang.xuan@ki.se
Topics
Preliminary findings SOM and PV.
- Regions of interest:
- Basal forebrain
- Thalamus.
- Septum.
- Amygdala.
- Hippocampus.
- Background and aims.
- Dual versus single rabies vector systems.
- Whole-brain reconstruction.
- Local versus long-range inputs
Background and Aims
(Carsten K Pfeffer et al., Nature Neuroscience, 2013)
- Retrograde tracing
- SAD B19G2
- Five genes
Rabies virus
Rabies-virus-glycoprotein (RVG) is necessary and sufficient for transsynaptic spread, but not for transcription or viral genome replication.
(Etessami et al., 2000, Mebatsion et al., 1996 and Wickersham et al., 2007)
- Avian EnvA-TVA
- Delivering TVA and RVG into starting cells
Cell-type-specific delivery
Dual vector system (traditional)
-
Starter cells definition
- True positive:
- + TVA-mCherry
- + Rabies-EGFP.
- + RVG
- False positives.
- + TVA-mCherry
- + Rabies-EGFP.
- - RVG
- True positive:
- Overestimation of starting population
- Not possible to dissect local input (e.g. between layers)
Leads to the following problems:
Pollak et al. 2014, Wall et al. 2013, Uchida et al. 2012
Dual vector system
- Tag RVG with fluorescent protein (e.g. EF1a-DIO-RVG-Venus).
Problem: RVG is sensitive to tag, miss-folding (pers. comm. Ed Callaway).
- All in one vector (e.g. EF1a-DIO-TVA-mCherry-t2A-RVG).
Problem: Too large to fit in standard vectors like AAV and lentivirus.
- One vector without tag (e.g. EF1a-DIO-TVA-t2A-RVG).
Problem: Not possible to know where primary infected cells are.
- Single vector rabies system. (e.g. EF1a-DIO-TVA-V5-t2A-RVG)
SOLUTION
Single vector system
V5 Paramyxovirus SV5
a small epitope present on the P and V proteins of SV5.
- 14 amino acids 42 bp.
- Works good with AAV vectors.
- Fusion protein with TVA on C-terminal membrane bound.
Local inputs
Single vector system
I've also extended the single vector rabies virus system with additional rabies varieties and flavors.
- Tracing: 3'-N-P-M-EGFP-L-5'.
- Gain of function: 3'-N-P-M-ChR2-mCherry-L-5'.
- Loss of function: 3'-N-P-M-Jaws-EGFP-L-5'.
- Input sensitivity: 3'-N-P-M-SSFO-EYFP-L-5'.
Disadvantage: toxicity of the rabies virus itself. Mechanism unknown.
Puts a limited time frame from injection to end-point of experiment.
Whole-Brain Reconstruction
Pollak Dorocic et al. 2014
Reconstructing brain from sectioned tissue
WholeBrain Web interface
similar to...
works with...
Local versus long-range input
- How much local versus long-range input.
- median spherical radial distance
Local versus long-range input
Local versus long-range input
- No marked difference between and .
- Statistical power issue.
This severely limits any quantitative comparison across all unique brain regions that cells were found in.
Until sample size is increased Qualitative findings
SOM
PV
Inputs from different brain areas
Cortical input
PV-cre mouse ID# 195
SOM-cre mouse ID# 80
~80% of all inputs are cortical input
Hippocampus-CA1, Stratum oriens
- ChAT
- Rabies-EGFP
Basal forebrain
- FOXP2
- PV
SOM-cre
PV-cre
Medial Septum
SOM-cre
PV-cre
Rabies-EGFP
ChAT
Amygdala
Ventral group of the dorsal thalamus
Summary
- Prefrontal cortex interneurons (PV and SOM) get more local inputs than long-range inputs.
- Prefrontal cortex interneurons (PV and SOM) get inputs mainly from cortical areas.
- Prefrontal cortex interneurons (PV and SOM) are heavily innervated by Cholinergic inputs from basal forebrain and pallidum (Globus pallidus)
- Prefrontal cortex interneurons (PV and SOM) are innervated by distinct parts of Amygdala, Thalamus and Hippocampus (CA1,2,3).
- No obvious differences found in between genotypes.
- Other interneurons (VIP)
- Principal cells (Coinjection with CaMKIIa-CRE)
- New vector designs: CaMKIIa-TVA-V5-t2A-RG
On-going work
- Marie Carlén
- Konstantinos Meletis
- Sofie Ährlund-Richter
- Daniel Fürth
- Xinming Wang
- Calvin Young
- Other members in the lab
Acknowledgement
Thank you!
Advantages and Disadvantages
- TVA-V5-RG Vs TVA-mCherry+RG(TVA-mCherry/non-RG infected cells)
- Local input
- •Disadvantages:
- Staining
- Alternative:
- AAV8/synP-FLEX-sTpEpB
- (Keigo Kohara et al., Nature Neuroscience 2014)
-
Reduction of total genome length by:
- using smaller promotor(human synapsin-1 promotor)
- using smaller polyadenylation signal(bovine growth hormone polyadenylation site)
-
removing all extraneous sequences and restriction sites
- 7 days+ 7 days
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