Title: Dyed Sand Lab Book
1Dyed Sand Lab Book
- Donna S. Lutz
- Iowa State University
- 2000
2COE Dyed Sand StudyMajor Objectives
- Use dyed sand to trace dredge material movement
in river system - Find appropriate dye to dye sand particles
- Develop fluorometry procedure to identify
presence of dyed sand - Evaluate the background interference caused by
chlorophyll
10/3/00
3Dayglo dyed sand
- Supplied by the COE
- 0.6 mm sand, 227g w/ 3.2 g dye
- Signal Green SG (534 nm)
- Saturn Yellow SY(563 nm)
- Rocket Red RR (614 nm)
- Horizon Blue HB(477 nm)
- nm are dominant transmittance / reflectance
supplied by Dayglo
10/3/00
410/3/00
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6Testing Solvents
- Prepared samples by dissolving 10 grains of 4
dyed sands in about 4.5 ml petroleum ether, 90
acetone, methylene chloride and water in 16x125mm
test tube. Each tube was inverted 50 times, then
vortex mixed for 15 sec. - Results, dye was soluble in acetone and methylene
chloride but not in water or petroleum ether
(These results were later confirmed by Dayglo)
10/3/00
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8Interference w/ chlorophyll
- Chlorophyll pigment extractions (90 actetone)
were examined under blue filter black light BLB
(St 1, 10 and 7 from Sayl 1248) - BLB wavelength 365nm (345-400nm)
- It was determined that chlorophyll does indeed
fluoresce in the red light spectrum - Main wavelength for chlorophyll is 630-665nm
- Recommend using dye outside this range
10/3/00
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10Preparation of Dyed Sand/Sand samples
- 2g 0.6mm sand with 0.1g of each of four dyes
added - Photo was taken under BLB of dry mixture
- Samples were dissolved in about 4.5 ml 90
acetone, inverted and mixed - BLB photo taken
10/3/00
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13Notes from 10/3/00
- HB dye may be a good choice, however trace fibers
also fluoresce blue - wavelength 477 is outside chlorophyll range
- it appears to fluoresce well
- Solvent could be acetone or methylene chloride
MeCl - Have ordered cells for Turner machine, should
arrive in 2-3 days
14To do next
- Will prepare chlorophyll sample using MeCl to
compare - Dyed Sand/Sand samples could be centrifuged to
remove turbidity - Will prepare Dyed Sand samples without the 2g
sand to compare - Will arrange to use spectrofluorometer to define
excitation and emmission filter selection for
Turner fluorometer
15Labwork 10/9/00
- Document lighting arrangement - COEs results are
brighter, either its our lighting or imaging - Investigate effect of centrifugation on turbidity
- Prepare samples of only 0.1g dyed sand with 90
acetone to compare to COE samples
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26Notes from 10/9/00
- COE lighting system is better
- Centrifuging at 3000 rpm for 10 min is adequate
to remove turbidity
27Work done 10/18/00 at Dr Jenks Lab
- 5 dye samples, chorophyll (St 7 from Week 1248),
acetone blank and sand/acetone blank were run - Scanning spectrophotometer was used to determine
excitation wavelength - Using determined excitation wavelength samples
were run on scanning spectrofluorometer - Dyed samples were dilute (20 drops from 0.1g dye
to 4.5ml acetone samples diluted to 3 ml) - Chlorophyll sample was not diluted
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33Initial Data 10/18/00
34Questions to Ask
- 1. Overall, what do the ISU spectrograms tell us?
- 2. What are the spectrograms from DayGlo and why
don't they match any of our results? - 3. Using a fluorometer, which dye would be the
most detectable (and distinguishable from
backgound, i.e. acetone, chlorophyll and sand)?
351. What do the spectrograms tell us?
- The spectrophotometer output shows us what the
excitation wavelength is for each sample. It is
assumed that if we excite the sample at its peak
excitation wavelength we will see the greatest
peaks in the spectrofluorometer output. - The scanning spectrofluorometer shows us at what
wavelength the sample fluoresces at, given that
specific excitation wavelength - The peaks seen in the photometry output are
mirrored with peaks in the fluorometry output, as
expected
361. What do the spectrograms tell us? (contd)
- Acetone gave a huge absorbance between 210 and
345 nm which was mirrored in the
spectrofluorometer results at 850 nm and above - Chlorophyll had two distinct peaks in absorbance
at 433 and 663 nm - Turbidity needs to be eliminated to reduce
noise/interference (see undyed sand-acetone
results) - Acetone blank will always have to be used and
acetone subtracted from results
372. What are the spectrograms from DayGlo and why
dont they match our data?
- Conference call 10/19 with N McVay, Corps and
Dick Bonsutton, DayGlo - DayGlo graphs are from a spectrophotometer using
dried paint samples - Measured parameter was reflectance
- Not considered strange that our dyed sand-acetone
samples would have different optical
characteristics
383. Using a fluorometer, which dye would be the
most detectable (and distinguishable from
backgound, i.e. acetone, chlorophyll and sand)?
- For best detection, the selected dye should have
an excitation wavelength outside of the range
210-345 nm, 620-675 nm and 400-500nm. Thus, HB,
RR and AP are candidates, however, HB may be a
little close to acetone. - HB has the sharpest fluorometer peak but it is
excitated near chlorophylls excitation
wavelength. - AP and RR appear to be good choices at this time.
39Comparison of Excitation Wavelengths
- RR and AP may be the best dyes to detect by
flluorometry because they excite at different
wavelengths than either acetone or cholorphyll
40What to do next?
- Return to Dr Jenks lab and
- Excite AP, chlorophyll and acetone at APs
excitation wavelength (555nm) and compare
spectrofluorograms - Excite RR, chlorophyll and acetone at RRs
excitation wavelength (527nm) and compare
spectrofluorograms - Excite HB, chlorophyll and acetone at HBs
excitation wavelength (365nm) and compare
spectrofluorograms - Explore if it is possible to select the emission
wavelength and scan the excitation wavelengths
412nd trip Dr Jenks Lab 10/23/00
- Samples were 10 dyed sand grains dissolved in 4.5
ml 90 acetone, acetone blank and chlorophyll
sample from St 1 for Sayl 1248 (undiluted) - Redid scans with spectrophotometer to verify
excitation wavelength for the dyes, AP, RR, and
HB. - Optical density from these samples was below the
optimum 0.1 to 0.3 range. - AP had the highest peaks on the spectrophotometer
scans, it was difficult to discern significant
peaks for HB. - Spectrophotometer scans revealed the same
excitation wavelength for AP (555 nm) and RR (530
nm).
42Spectrofluorograms from 10/23/00
- Excited AP, chlorophyll and acetone at APs
excitation wavelength (555nm) and compared
spectrofluorograms AP peaks are different than
acetone but are masked by chlorophyll - Excited RR, chlorophyll and acetone at RRs
excitation wavelength (530nm) and compared
spectrofluorograms RR peaks are different than
acetone but are masked by chlorophyll - Excite HB, chlorophyll and acetone at HBs
possible excitation wavelengths (370nm and 730
nm) and compared spectrofluorograms no good HB
detection at 730nm, but there could be far end
(gt790nm) peak for HB that would be
distinguishable. - Was told it was not advisable to select the
emission wavelength and scan the excitation
wavelengths on the fluorometer that the
spectrophotometer would give better results.
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45Conclusions from 2nd lab Jenks lab study
- AP has highest optical density of the samples,
which may mean greater detection and it is easily
distinguished from acetone - However, chlorophyll can block all dyes at their
excitation wavelengths. - Will need to minimize chlorophyll contamination
in the sample before dissolving dye in order to
measure spectrally.
46What to do next?
- Might be worth taking one more look at HB and
extend the scan to the maximum 880 nm - Then the focus should be on how to reduce the
effect of chlorophyll - physically remove chlorophyll through sample
preparation - mechanically shake, rinse samples, dry,
centrifuge and filter? - If the Corps wants to pursue this avenue further,
wed want real samples from the river with
undyed sand and dyed sand (AP or RR).