Beauchamp:NIRS

Eswen Fava's NIRS Manual

Probe Creation:

• 3.2cm from source to detector (note absorption is 2/3 the distance of source to detector)
• [Munster T2T-Converter (3D Version)[1]] (does not open in new window!)

• Tools that are helpful:
• simple: compass, superglue (with brush), hand single hole punch, drill bit to go through plastic
• speciality: face-lift compression garments, scuba caps, soccer header headband (temporal probe),
• online vendors: McMaster-Carr - nylon machine screws, panhead 1/4" in length

Experimental Design:

• Keep in mind Hemodynamic Response Function properties when designing an experiment using NIRS
• e.g., Infant experiments (Bortfeld, Fava & Boas 2009) duration of baselines: 10 seconds, duration of stimuli: 20 seconds
• horizontal axis: time in seconds,
• vertical axis: percent increase in MR signal due to the BOLD effect.

Hemodynamic Function (HRF):

• After the onset of the stimulus, a small decrease in MR signal is observed, caused by the fact that oxygen from the blood is used, but that the blood supply is not yet altered. This makes that the concentration deoxyhemoglobin rises and that the MR signal is more disturbed.
• Shortly after this initial dip, the signal rapidly begins to rise due to the supply of more and more oxygenated blood. There is more supply of oxygenated blood than is necessary and this gives an increased MR signal till the end of the stimulus. A few seconds after the end of the stimulus the signal rapidly decreases to end, via a post-stimulus undershoot, at its normal level.
• The post-stimulus undershoot is caused by the fact that the cerebral blood flow is more locked to stimuli than is the cerebral blood volume. The resulting increase in blood volume leads to a decrease in MR signal. Picture is obtained and adapted from the website of Radiopaedia [79].
• To find the small increase in MR activity due to the stimulus, usually the General Linear Model (GLM) is used. With this method the activity due to the presented stimulus is modelled by convolving the time-course of the stimulus presentation with the hemodynamic response function. In the next step the correlation between the model and the time course of the MR signal at each voxel or region is calculated by using linear regression. The result is a regression coefficient (r) and a p-value for each voxel or region. The p-value indicates how likely it is that the correlation between the GLM and the time course of the signal can be explained by chance instead of the stimulus."

[Taken from mst.nl http://www.mst.nl/neurochirurgie/Onderzoek/tinnitus.doc

Checking Laser Reading Power Levels: (Note: you CANNOT see 830nm, you CAN see 690nm (appears red))

• all lasers of same wavelength should be in the same range (e.g., all 690 lasers should be between 13.01 and 13.9)
• adjust lasers with small screwdriver.

• when using power meter to measure from the laser
• 690nm should read at 13mW or 12.5mW
• 830nm should read at 10mW

• when using power meter to measure from the probe end of your fibers, expect your fibers to lose between 30 and 50% of the light
• 690nm should be about 8.45
• 830nm should be about 6.45

Checking your Fibers:

• If you move your fibers around a lot, or exchange one set for another consider frequently checking them once per month

• You can also check your fibers by holding the laser end up to an incandescent bulb and holding the emitter’s probe end to the wall. The light should form a whole circle.
• Be sure to look at 1 wavelength at a time

• When you receive new fibers, hook them up to the 690nm lasers and hold them up to the wall to check for the whole circle pattern
• If you don’t see that pattern, epoxy or broken fiber optics could be to blame. Send them back!

Checking your Emitters (see picture at right):

• Turn Laser 1 ON (690nm)
• Turn all other Lasers OFF
• Probe ends of fibers are facing a wall
• Remove fiber from Laser 1 690 source - watch for any changes in amplitude or signal quality for detectors 1&2
• Repeat for all source-detector pairs (be sure to turn ON the laser you want to investigate, and OFF the remaining lasers)

Checking your Detectors (see picture at right):

• Turn ON all lasers
• Unplug ALL detectors
• Plug in detectors one at a time and note any changes in the amplitude or signal quality change

Checking to see which Detectors your Sources go to:

1. Use a phantom head, or wrap a blanket in a tight ball
2. Put probe on phantom
3. Turn ON a source (e.g., turn on Laser 1)
4. With a source on, REMOVE detectors 1 by 1 (leave the previous detectors unplugged as you continue) - note any changes in movement, or lack of movement from the detectors.
5. Note if pre-clipping gain light is on or not for each of the detectors
6. Plug all detectors back IN, turn OFF source 1, Repeat steps 3 and 5, cycling through your sources. Continue this process until you have gone through all of your sources.

Checking to see which Sources your Detectors go to:

1. Use a phantom head, or wrap a blanket in a tight ball
2. Put probe on phantom
3. Turn ON all sources (e.g., turn on Lasers 1, 2, 3, 4)
4. With all sources on, REMOVE only detector 1
5. Note any changes in movement, or lack of movement from the remaining plugged in detectors as you do this
6. Note if pre-clipping gain light is on or not for each of the detectors
7. Make sure all detectors are plugged IN, keep ALL sources ON, repeat steps 3 through 5, cycling through your detectors. Continue this process until you have gone through all of your detectors.