A simple single cell model#
Building and testing detailed models of individual cells, then optimizing their parameters is usually the first step in building models with multi-compartment cells. Arbor supports a single cell model workflow for this purpose, which is a good way to introduce Arbor’s cell modelling concepts and approach.
Note
Concepts covered in this example:
The Arbor library and units.
Intro to morphologies.
Intro to region and locset expressions.
Intro to decors and cell decorations.
Building a
arbor.cable_cellobject.Building a
arbor.single_cell_modelobject.Running a simulation and visualising the results.
Setup and introduction to units#
We begin by importing the Arbor library and its unit support.
import arbor as A
from arbor import units as U
As we will refer to both quite often, we assign aliases A and U, to
minimize typing. Over the course of this introduction, you will notice that most
of Arbor’s user interface is making use of units. This requires a bit of typing,
but makes the physical quantities obvious and allows for easy conversion of
models. You can use any sensible unit for a given dimension and Arbor will
convert as needed, e.g. you can write 5 * U.mm instead of 5000 * U.um.
Handing a mismatching dimension to a method will cause a runtime error, so in
the example above, 5 * U.mV will be rejected.
The cell#
The most trivial representation of a cell in Arbor is to model the entire cell as a single cylinder. The following example shows the steps required to construct a model of a cylindrical cell with a length of 6 μm and a radius of 3 μm; Hodgkin–Huxley dynamics and a current clamp stimulus, then run the model for 30 ms.
The first step is to construct the cell. In Arbor, the abstract representation
used to define a cell with branching cable morphology is a cable_cell, which
holds a description of the cell’s morphology, named regions and locations on the
morphology, and descriptions of ion channels, synapses, threshold detectors and
electrical properties. We will go over these one by one.
Our cell has a simple morphology comprising a single segment, which is why we use an explicit construction. Normally, one would read the morphology from file and Arbor handles most standard formats natively.
# (1) Create a morphology with a single (cylindrical) segment of length=diameter=6 μm
tree = A.segment_tree()
tree.append(A.mnpos, A.mpoint(-3, 0, 0, 3), A.mpoint(3, 0, 0, 3), tag=1)
This constructs a arbor.segment_tree (see also segment
tree) containing a single segment. You can skip the rest of
this paragraph on first reading, it explains the details of constructing a
morphology from scratch. The segment tree is the representation used to
construct the morphology of a cell. A segment is a tapered cone with a tag; the
tag can be used to classify the type of the segment (for example soma, dendrite
etc). To create a segment tree representing our single-cylinder cell, we need to
add one segment to our tree object. We use the
arbor.segment_tree.append() method, which takes 4 arguments: the parent
segment which does not exist for the first segment, so we use
arbor.mnpos; the proximal arbor.mpoint (location and radius)
of the segment; the distal arbor.mpoint of the segment; and the tag.
# (2) Define the soma and its midpoint
labels = A.label_dict({"soma": "(tag 1)", "midpoint": "(location 0 0.5)"})
Next, we create a dictionary of labels
(arbor.label_dict) to assign properties to. This is a
handy tool to connect part of your morphology to semantically meaningful names.
Labels give names to regions and location
described using a DSL based on s-expressions. Labels from the dictionary can
then be used to facilitate adding synapses, dynamics, stimuli and probes to the
cell. We add two labels:
somadefines a region with(tag 1). Note that this corresponds to thetagparameter that was used to define the single segment in step (1).midpointdefines a location at(location 0 0.5), which is the mid point0.5of branch0, which corresponds to the midpoint of the soma on the morphology defined in step (1).
# (3) Create and set up a decor object
decor = (
A.decor()
.set_property(Vm=-40 * U.mV)
.paint('"soma"', A.density("hh"))
.place('"midpoint"', A.iclamp(10 * U.ms, 2 * U.ms, 0.8 * U.nA), "iclamp")
.place('"midpoint"', A.threshold_detector(-10 * U.mV), "detector")
)
The final piece constructs a arbor.decor describing the distribution
and placement of dynamics and properties on a cell. The cell’s default
properties can be modified, and we can use arbor.decor.paint() and
arbor.decor.place() to further customise it in the following way:
arbor.decor.set_property()is used to set some default properties on the entire cell. In the above example we set the initial membrane potential to -40 mV.arbor.decor.paint()is used to set properties or add dynamics to a region of the cell. We call this method ‘painting’ to convey that we are working on sections of a cell, as opposed to precise locations: for example, we might want to paint a density ion channel on all dendrites, and then place a synapse at the tip of the axon. In the above example we paint HH dynamics on the region we previously named"soma"in our label dictionary.arbor.decor.place()is used to add objects on a precisearbor.locationon a cell. Examples of objects that are placed are synapses, threshold detectors, current stimuli, and probes. In the above example we place a current stimulusarbor.iclampwith a duration of 2 ms and a current of 0.8 nA, starting at 10 ms on the location we previously labelled"midpoint". We also place aarbor.threshold_detectorwith a threshold of -10 mV on the same location.
# (4) Create cell and the single cell model based on it
cell = A.cable_cell(tree, decor, labels)
The three ingredients – morphology, labels, and decor – are joined into a cable cell.
The single cell model#
Once the cell description has been built, the next step is to build and run the
simulation. Arbor provides an interface for constructing single cell models with
the arbor.single_cell_model helper that creates a model from a cell
description, with an interface for recording outputs and running the simulation.
# (5) Make single cell model.
m = A.single_cell_model(cell)
The single cell model has 4 main functions:
It holds the global properties of the model
It registers probes on specific locations on the cell to measure the voltage.
It runs the simulation.
It collects spikes from threshold detectors and voltage traces from registered probes.
Right now, we’ll only set a probe. The model is complete without, but to see the results, we need to extract some data.
# (6) Attach voltage probe sampling at 10 kHz (every 0.1 ms).
m.probe("voltage", '"midpoint"', tag="Um", frequency=10 * U.kHz)
Note, that the probe is given a location from the label dictionary midpoint,
the value to record voltage, the sampling frequency, and finally a tag by
which we can reference it later, here Um.
Now, we can start the actual simulation:
# (7) Run simulation for 30 ms of simulated activity.
m.run(tfinal=30 * U.ms)
The results#
Our cell and model have been defined and we have run our simulation. Now we can look at the resulting spikes and membrane potential.
# (8) Print spike times.
print("{} spikes:".format(len(m.spikes)))
for s in m.spikes:
print(f" * {s:3.3f} ms")
To print the spike times, we use arbor.single_cell_model.spikes(). A
single spike should be generated at around the same time the stimulus we
provided in step (3) gets activated (10ms).
And, finally, we plot the membrane potential
# (9) Plot the recorded voltages over time.
print("Plotting results ...")
sns.set_theme() # Apply some styling to the plot
df = pd.DataFrame({"t/ms": m.traces[0].time, "U/mV": m.traces[0].value})
sns.relplot(data=df, kind="line", x="t/ms", y="U/mV", errorbar=None).savefig(
"single_cell_model_result.svg"
)
We should be seeing something like this:
Plot of the potential over time for the voltage probe added in step (6).#
The full code#
You can find the source code for this example in full at
python/examples/single_cell_model.py which comes in at roughly 10 lines of
Python to define and simulate a cell from scratch.