1. General Discussion:
1.1 Collection Procedure:
The sample is drawn through
a cassette containing a FWSB filter for the collection of particulate
phosphorus pentasulfide.
1.2 Analytical Procedure:
The
collected phosphorus pentasulfide is extracted by the mixture of sodium
hydroxide and hydrogen peroxide based on the following proposed reaction
and analyzed by ion chromatography (IC) as phosphate and sulfate ions.
P2S5 + 20H202 +
160H-1 = 2PO4-3 +
5SO4-2 + 28H20 2. Range and
Detection Limit:
2.1 The range is from 1.25 to 2,500 µg phosphate. This
corresponds to either 1.5 to 3,000 µg phosphorus pentasulfide or 0.025
to 6.25 mg/m³ of phosphorus pentasulfide for a 60 to 480 L air volume at
a flow rate of 1 Lpm, respectively.
2.2 The quantitative
detection limit is 0.01 µg of phosphate per injection or 1.5 µg of
phosphorus pentasulfide in a 25 mL sample volume for a 200 µL sample
injection volume. This corresponds to 0.025 mg/m³ of phosphorus
pentasulfide for a 60 L air volume at a flow rate of 1 Lpm for 60
minutes. 3. Precision and Accuracy:
The precision and
accuracy have not been completely determined this time, but the
preliminary study has shown that the coefficients of variation for
analytical method in terms of phosphate were between 0.0055 and 0.058 in
the range of 24 to 34 µg/mL and in terms of sulfate were between 0.023 and
0.047 in the range of 62 to 87 µg/mL.
4. Interferences:
4.1 If both phosphate and sulfate are present in the
atmosphere, they would give a positive interference; otherwise, either
one of them causes no serious interference.
4.2 Any ionic
substance that would elute at the same retention time as phosphate and
sulfate would be a positive interference.
4.3 When other
substances are known or suspected to be present in the air, such
information, including their suspected identities, should be transmitted
with the sample. Substances, such as phosphoric acid and all kinds of
phosphorus compounds, etc, may interfere with the determination of
phosphate.
4.4 It has been reported (11.1, 11.2) that phosphorus
pentasulfide may decompose upon exposure to moist air or moisture to
form phosphoric acid and hydrogen sulfide. This may result in the low
recovery of phosphorus pentasulfide based on only the sulfate
determination. 5. Advantage and Disadvantage:
5.1 With the proper selection of instrumental conditions and
conductivity range, this method has adequate sensitivity for measuring
workplace atmosphere concentrations of phosphorus
pentasulfide.
5.2 Although it is not required, the method can be
fully automated.
5.3 The amount of phosphorus pentasulfide may be
simultaneously confirmed from both phosphate and sulfate ions formed
during the sample determination.
5.4 One disadvantage is that no
information is available so far for the sampling procedure due to the
lack of aerosol generation system. However, this problem can be solved
in the future. 6. Apparatus:
6.1 Ion chromatograph: Dionex 10 or equivalent.
6.2
Auto sampler: WISP Model 710A or equivalent.
6.3 WISP auto
sampler containers, including 4 mL vials, caps and septums.
6.4
Recorder: Varian Model 9176 or equivalent.
6.5 Anion precolumn,
anion separator column and anion suppressor column.
6.6 Timer:
Universal timer or equivalent.
6.7 Vacuum filtration apparatus.
6.8 Membrane filters, 5.0 µm pore size, 37mm diameter (MSA FWSB
or equivalent)
6.9 Miscellaneous assorted laboratory glassware:
beakers, pipettes, volumetric flasks, etc. (Note: All glassware should
be washed in "phosphate-free" detergent and rinsed thoroughly with
deionized water and then air-dried prior to use.)
6.10 Hot
plate. 7. Reagents:
All chemicals should be ACS
reagent grade or equivalent.
7.1 Sodium carbonate, anhydrous
7.2 Sodium
bicarbonate
7.3 Strong eluent (0.003 M sodium bicarbonate/0.006 M
sodium carbonate): Dissolve 1 g of sodium bicarbonate and 2.5 g of
sodium carbonate and dilute to a 4 L volume with deionized
water.
7.4 Sulfuric acid, concentrated (98%)
7.5 Anion
regenerant solution, 1N sulfuric acid: Slowly dilute 111 mL of
concentrated sulfuric acid to 4 L with deionized water.
7.6
Sodium sulfate, anhydrous
7.7 Sulfate stock standard (1,000 ppm
sulfate): Dissolve and dilute 1.4792 g of sodium sulfate to 1 L with
deionized water.
7.8 Potassium dihydrogen phosphate, anhydrous
7.9 Phosphate stock standard (1,000 ppm phosphate): Dissolve and
dilute 1.389 g of anhydrous potassium dihydrogen phosphate to 1 L with
deionized water.
7.10 Sodium hydroxide, 5 N: Dissolve 200 g of
sodium hydroxide pellets in approximately 600 mL of deionized water and
dilute to 1 L.
7.11 Hydrogen peroxide, 3%: Dilute 10 mL of 30%
hydrogen peroxide to 100 mL with deionized water. 8. Proposed
OSHA Collection Procedure:
8.1 Apparatus:
8.1.1 Personal sampling pump.
8.1.2 Filter
cassettes: A 37 mm diameter FWSB filter contained in a 37-mm
polystyrene two piece cassette filter holder. 8.2
Procedure:
8.2.1 Sampling is done in accordance with instructions
contained in the IHFOM (or the Industrial Hygiene Technical Manual
when available to the OSHA industrial hygienist).
8.2.2
Collect each sample with a 5.0 µm FWSB filter at a known flow rate of
1 L/min. A minimum air volume of 120 L is recommended.
9. Analytical Procedure:
9.1 Sample preparation:
9.1.1 Rinse all glassware with deionized water. Commercial
detergents containing phosphate should not be used.
9.1.2
Remove the filter from the cassette and place in a clean 125-mL
conical beaker.
9.1.3 Pipette 1 mL of 5 N NaOH into each
conical beaker and let stand, with occasional vigorous shaking for 30
minutes.
9.1.4 Add 2 mL of 3% hydrogen peroxide into each
sample and let stand for a while.
9.1.5 Add 5 mL of deionized
water and cover with watchglass. Heat to boiling for 5 minutes.
9.1.6 Cool to room temperature and transfer each sample to 25
mL volumetric flask and dilute to the mark with deionized water.
9.1.7 Filter the sample solution by means of the vacuum
filtration apparatus.
9.1.8 If an auto sampler is to be used
in the analysis, transfer a portion of each sample filtrate to an auto
sampler vial. A minimum volume of 1.5 mL is required in each auto
sampler vial.
9.1.9 If manual injection is to be used in the
analysis, quantitatively transfer each sample filtrate to a clean
glass 20 mL vial.
9.1.10 Be sure to label each vial with the
appropriate laboratory ID number. 9.2 Standard Preparation:
9.2.1 Prepare a series of mixtures of phosphate and
sulfate standards in the ratio of 1:2, respectively, by making
appropriate serial dilutions of the 1,000 ppm phosphate and sulfate
stock solution with the strong eluent.
9.2.2 If an auto
sampler is to be used in the analysis, fill the auto sampler vials
with appropriate standard solutions. 9.3 Analysis:
9.3.1 Typical operating conditions are:
Eluent:
0.003 M sodium bicarbonate/0.006 M sodium carbonate
Precolumn:
3-mm × 50-mm anion
Separator column: 3-mm × 250-mm
anion
Suppressor column: 6-mm × 100-mm anion
Column
temperature: Ambient
Conductivity meter: 10 or 30 µMHO full
scale
Pump setting: 20-25% of total capacity
Retention
time: Approximately 9 minutes for phosphate and 19 minutes for
sulfate.
9.3.2 Set up the dual pen recorder an two different
full-scale ranges (typically 200 and 500 mv).
9.3.3
Equilibration: Allow the IC columns to equilibrate by pumping the
eluent through the system for a least one hour before analysis or
until a stable baseline is achieved.
9.3.4 Auto sampler:
9.3.4.1 If an auto sampler is used in the analysis,
place the standard and sample auto sampler vials in the carriage.
Use the Sample Identification Record Sheet to identify each standard
and sample.
9.3.4.2 Check the operation manual to select the
appropriate programming mode.
9.3.4.3 Set the timer for
controlling the recorder and ion chromatograph. Start the auto
sampler. 9.3.5 Manual injection: Inject the standard or
sample into the 100 µL sample loop of the ion chromatograph with a 1mL
syringe. It is advisable to inject a sample volume of at least three
times the sample loop volume to ensure adequate rinsing of the loop
from sample contamination and to prevent standard carryover. Rinse the
syringe several times with deionized water between sample injections.
9.3.6 Observe the first few standard chromatograms to ensure
proper operation. Periodically, check the zero offset between samples
to detect and correct any baseline drift and ensure proper
sensitivity.
9.3.7 Analyze the standards and samples under the
same operation conditions and time period to monitor the performance
of the analytical system. Check the retention times of the standards
and samples to ensure uniformity as the analysis proceeds.
9.3.8 Analyze a series of standards in the range of interest
at concentrations about 25% above and below the apparent sample
concentrations.
9.3.9 Establish positive identity of the
phosphate and sulfate peaks by adding known amounts of standard
solutions if interfering substances are present.
9.3.10
Measure the peak heights of phosphate and sulfate of the samples and
standards in millimeters.
9.3.11 Use the Auto Colorimetric or
any available least square regression program to establish calibration
curves of peak heights vs. the amount of phosphate and sulfate in the
standards in units of µg or µg/mL. 10.
Calculations:
10.1 Read the sample weight as phosphate and as sulfate in
µg from the calibration curves (see Section 9.3.11).
10.2 Make a
blank correction, if necessary, as follows:
|
W
|
= (A - B)×V×G
|
| Where: |
W |
= Corrected amount (µg) of phosphorus
pentasulfide in the sample solution. |
|
A |
= Amount (µg/mL) as phosphate or as
sulfate found in the sample solution. |
|
B |
= Amount (µg/mL) as phosphate or as
sulfate found in the blank sample solution. |
|
V |
= Sample volume (mL) = 25 mL |
|
G |
= Gravimetric factors = 1.17 for phosphate
and 0.463 for sulfate |
10.3 The corrected
amount of phosphorus pentasulfide (W) calculated from both phosphate and
sulfate peaks should be in agreement within plus and minus 10%.
Otherwise, the lower amount, W, should be used for calculating the
concentration of phosphorus pentasulfide in air (see next section).
10.4 The concentration of phosphorus pentasulfide in the air
sample is expressed in mg/m³, which is numerically equal to µg/L.
mg/m³ = [W (from Sec.10.2 and 10.3),µg]/(Air sampled vol., L)
11. References:
11.1 The Condensed Chemical Dictionary, 8th Ed.,1971
11.2 The Merck Index, 9th Ed., Published by Merch and Co., Inc.
Rahway, N.J.
| Table 1 |
Purity of Phosphorus
Pentasulfide(1)
|
| Weight of Phosphorus Pentasulfide:
632.15 mg |
| Solution Volume: 500 mL |
| Theoretical Concentrations: |
1080.8 µg/mL as
Phosphate
2730.5 µg/mL as Sulfate
|
| Sample No. |
Phosphate Found, µg/mL |
Sulfate Found, µg/mL |
| |
| 1 |
1030.3 |
2733.4 |
| 2 |
1030.3 |
2591.8 |
| 3 |
1020.5 |
2492.2 |
| |
| n = |
3 |
3 |
| mean = |
1027.0 |
2605.8 |
| SD = |
5.7 |
121.2 |
| CV1 = |
0.0055 |
0.047 |
| Purity = |
95.0% |
95.4% |
| |
| (1) P1316, Eastman, Lot No. 671-1X,
Practical |
| Table 2 |
| Independent Method |
IC vs. NIOSH Colorimetric
for Phosphate
|
| Sample No. |
Wt. of P2S5, mg |
P2S5 Found, mg |
P2S5 Recovery, % |
|
|
|
|
|
|
| |
|
IC |
Color. |
IC |
Color. |
|
|
|
|
| 1 |
31.62 |
27.75 |
25.41 |
87.8 |
80.4 |
| 3 |
40.17 |
32.46 |
32.13 |
80.8 |
80.0 |
| 3 |
56.91 |
44.81 |
29.19(1) |
78.6 |
51.2(1) |
| |
|
|
|
|
|
| |
|
|
n = |
3 |
2 |
| |
|
|
Mean = |
82.4 |
80.2 |
| |
|
|
SD = |
4.8 |
0.28 |
| |
|
|
CV1 |
0.058 |
0.0035 |
| |
| (1) Sample lost during anlysis, excluded
from statistical analysis. |
| Reference: P and CAM 216 and No.S333
NIOSH Methods. |
|
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