Melt a quantity of the substance slowly, while stirring, until it reaches a temperature of 90° or higher to completely melt the substance. Remove the source of heat, and allow the molten substance to cool to a temperature of 8 to 10° above the expected melting point. Chill the bulb of an ASTM 14C (American Society for Testing and Materials) or equal thermometer to 5°, wipe it dry and while it is still cold dip into the molten substance so that approximately the lower half of the bulb is submerged. Withdraw it immediately, and hold it vertically away from the heat until the wax surface dulls, then dip it for 5 min into a water bath having a temperature not higher than 16°.
Fix the thermometer securely in a test tube so that the lower point is 15 mm above the bottom of the test tube. Suspend the test tube in a water bath adjusted to about 16°, and raise the temperature of the bath a the rate of 2° per min to 30°, then change to a rate of 1° per min and note the temperature at which the first drop of melted substance leaves the thermometer. Repeat the determination twice on a freshly melted portion of the sample. If the variation of three determinations is less than 1°, take the average of the three as the melting point. If the variation of the three determinations is greater than 1°, make two additional determinations and take the average of the five.
“Carbon number” is number of carbon atoms in a molecule. Determine the carbon number distribution of the sample using the method as described in ASTM D 5442.
NOTE: By optimizing the length of separation column and/or column temperature, waxes with carbon number higher than 45 can also be included.
The combined contents of components with carbon number less than 25 is not more than 5%.
Using the carbon number distribution obtained in the test for “Carbon number at 5% distillation point” calculate the average molecular weight by the following formula:
where
i = the carbon number Ci is the content in % of components having a carbon number of i
General Instructions
Because of the sensitivity of the test, the possibility of errors arising from contamination is great. It is of the greatest importance that all glassware be scrupulously cleaned to remove all organic matter such as oil, grease, detergent residues, etc. Examine all glassware, including stoppers and stopcocks, under ultraviolet light to detect any residual fluorescent contamination. As a precautionary measure it is a recommended practice to rinse all glassware with purified isooctane immediately before use. No grease is to be used on stopcocks or joints. Great care to avoid contamination of wax samples in handling and to assure absence of any extraneous material arising from inadequate packaging is essential. Because some of the polynuclear hydrocarbons sought in this test are very susceptible to photo-oxidation, the entire procedure is to be carried out under subdued light.
Apparatus
– Separatory funnels: 250-ml, 500-ml, 1,000-ml, and preferably 2000-ml capacity, equipped with tetrafluoroethylene polymer stopcocks.
– Reservoir: 500-ml capacity, equipped with a 24/40 standard taper male fitting at the bottom and a suitable balljoint at the top for connecting to the nitrogen supply. The male fitting should be equipped with glass hooks.
– Chromatographic tube: 180 mm in length, inside diameter to be 15.7 mm ± 0.1 nun, equipped with a coarse, fritted-glass disc, a tetrafluoroethylene polymer stopcock, and a female 24/40 standard tapered fitting at the opposite end. (Overall length of the column with the female joint is 235 mm). The female 24/40 standard tapered fitting at the opposite end.
– Disc: Tetrafluoroethylene polymer 2-inch diameter disc approximately 3/16-inch thick with a hole bored in the center to closely fit the stem of the chromatographic tube.
– Heating jacket: Conical, for 500-ml separatory runnel. (Used with variable transformer heat control).
– Suction flask: 250-ml or 500-ml filter flask.
– Condenser: 24/40 joints, fitted with a drying tube, length optional.
– Evaporation flask (optional): 250-ml or 500-ml capacity all-glass flask equipped with standard taper stopper having inlet and outlet tubes permitting passage of nitrogen across the surface of the liquid to be evaporated.
– Vacuum distillation assembly: All glass (for purification of dimethyl sulfoxide); 2 litre distillation flask with heating mantle; Vigreaux vacuum-jacketed condenser (or equivalent) about 45 cm in length and distilling head with separable cold finger condenser. Use of tetrafluoroethylene polymer sleeves on the glass joints will prevent freezing. Do not use grease on stopcocks or joints.
– Spectrophotometric cells: Fused quartz cells, optical path length in the range of 5.000 ± 0.005 cm; also for checking spectrophotometer performance only, optical path length in the range 1.000 ± 0.005 cm. With distilled water in the cells, determine any absorbance differences.
– Spectrophotometer: Spectral range 250-400 nm with spectral slit width of 2 nm or less, under instrument operating conditions for these absorbance measurements, the spectrophotometer shall also meet the following performance requirements:
– Nitrogen cylinder: Water-pumped or equivalent purity nitrogen in cylinder equipped with regulator and valve to control flow at 5 p.s.i.g.
Reagents and materials
– Organic solvents: All solvents used throughout the procedure shall meet the specifications and tests described in this specification. The isooctane, benzene, acetone, and methyl alcohol designated in the list following this paragraph shall pass the following test:
To the specified quantity of solvent in a 250-ml Erlenmeyer flask, add 1 ml of purified n-hexadecane and evaporate on the steam bath under a stream of nitrogen (a loose aluminium foil jacket around the flask will speed evaporation). Discontinue evaporation when not over 1 ml of residue remains. (To the residue from benzene add a 10 ml portion of purified isooctane, re-evaporate, and repeat once to insure complete removal of benzene).
Alternatively, the evaporation time can be reduced by using the optional evaporation flask. In this case the solvent and n-hexadecane are placed in the flask on the steam bath, the tube assembly is inserted, and a stream of nitrogen is fed through the inlet tube while the outlet tube is connected to a solvent trap and vacuum line in such a way as to prevent any flow-back of condensate into the flask.
Dissolve the 1 ml of hexadecane residue in isooctane and make to 25 ml volume. Determine the absorbance in the 5 cm path length cells compared to isooactane as reference. The absorbance of the solution of the solvent residue (except for methyl alcohol) shall not exceed 0.01 per cm path length between 280 and 400 nm. For methyl alcohol this absorbance value shall be 0.00.
– Isooctane (2,2,4-trimethylpentane): Use 180 ml for the test described in the preceding paragraph. Purify, if necessary, by passage through a column of activated silica gel, grade 12, Davison Chemical Company, Baltimore, Maryland, USA, or equivalent, about 90 cm in length and 5 cm to 8 cm in diameter.
– Benzene, reagent grade: Use 150 ml for the test. Purify, if necessary, by distillation or otherwise.
– Acetone, reagent grade: Use 200 ml for the test. Purify, if necessary, by distillation.
– Eluting mixtures:
1. 10% benzene in isooctane: Pipet 50 ml of benzene into a 500-ml glass-stoppered volumetric flask and adjust to volume with isooctane, with mixing.
2. 20% benzene in isooctane: Pipet 50 ml of benzene into a 250-ml glass-stoppered volumetric flask, and adjust to volume with isooctane, with mixing.
3. Acetone-benzene-water mixture: Add 20 ml of water to 380 ml of acetone and 200 ml of benzene, and mix.
– n-Hexadecane, 99% olefin-free: Dilute 1.0 ml of n-hexadecane to 25 ml with isooctane and determine the absorbance in a 5-cm cell compared to isooctane as reference point between 280-400 nm. The absorbance per centimeter path length shall not exceed 0.00 in this range. Purify, if necessary, by percolation through activated silica gel or by distillation.
– Methyl alcohol, reagent grade: Use 10.0 ml of methyl alcohol. Purify, if necessary, by distillation.
– Dimethyl sulfoxide: Pure grade, clear, water-white, m.p. 18° minimum. Dilute 120 ml of dimethyl sulfoxide with 240 ml of distilled water in a 500-ml separatory funnel, mix and allow to cool for 5-10 min. Add 40 ml of isooctane to the solution and extract by shaking the funnel vigourously for 2 min. Draw off the lower aqueous layer into a second 500-ml separatory funnel and repeat the extraction with 40 ml of isooctane. Draw off and discard the aqueous layer. Wash each of the 40-ml extracts three times with 50 ml portions of distilled water. Shaking time for each wash is 1 min. Discard the aqueous layers. Filter the first extract through anhydrous sodium sulfate pre-washed with isooctane (see Sodium sulfate under “Reagents and Materials” for preparation of filter), into a 250-ml Erlenmeyer flask, or optionally into the evaporating flask. Wash the first separatory funnel with the second 40-ml isooctane extract, and pass through the sodium sulfate into the flask. Then wash the second and first separatory funnels successively with a 10 ml portion of isooctane, and pass the solvent through the sodium sulfate into the flask. Add 1 ml of n-hexadecane and evaporate the isooctane on the steam bath under nitrogen. Discontinue evaporation when not over 1 ml of residue remains. To the residue, add a 10 ml portion of isooctane and re-evaporate to 1 ml of hexadecane. Again, add 10 ml of isooctane to the residue and evaporate to 1 ml of hexadecane to insure complete removal of all volatile materials. Dissolve the 1 ml of hexadecane in isooctane and make to 25 ml volume. Determine the absorbance in 5 cm path length cells compared to isooctane as reference. The absorbance of the solution should not exceed 0.02 per cm path length in the 280-400 nm range. (Note – Difficulty in meeting this absorbance specification may be due to organic impurities in the distilled water. Repetition of the test omitting the dimethyl sulfoxide will disclose their presence. If necessary to meet the specification, purify the water by redistillation, passage through an ion-exchange resin, or otherwise).
Purify, if necessary, by the following procedure: To 1.5 litre of dimethyl sulfoxide in a 2-litre glass-stoppered flask, add 6.0 ml of phosphoric acid and 50 g of Norit A (decolorizing carbon, alkaline) or equivalent. Stopper the flask, and with the use of a magnetic stirrer (tetrafluoroethylene polymer coated bar) stir the solvent for 15 min. Filter the dimethyl sulfoxide through four thicknesses of fluted paper (18.5 cm), Schleicher & Schuell No. 597, or equivalent. If the initial filtrate contains carbon fines, refilter through the same filter until a clear filtrate is obtained. Protect the sulfoxide from air and moisture during this operation by covering the solvent in the funnel and collection flask with a layer of isooctane. Transfer the filtrate to a 2-litre separatory funnel and draw off the dimethyl sulfoxide into the 2-litre distillation flask of the vacuum distillation assembly and distill at approximately 3-mm Hg pressure or less. Discard the first 200-ml fraction of the distillate and replace the distillate collection flask with a clean one.
Continue the distillation until approximately 1 litre of the sulfoxide has been collected.
At completion of the distillation, the reagent should be stored in glass-stoppered bottles since it is very hygroscopic and will react with some metal containers in the presence of air.
Phosphoric acid, 85% reagent grade
– Sodium borohydride, 98%
– Magnesium oxide (Sea Sorb 43, Food Machinery Company, Westvaco Division distributed by chemical supplier firms, or equivalent): Place 100 g of the magnesium oxide in a large beaker, add 700 ml of distilled water to make a thin slurry, and heat on a steam bath for 30 min with intermittent stirring. Stir well initially to insure that all the absorbent is completely wetted. Using a Buchner funnel and a filter paper of suitable diameter, filter with suction. Continue suction until water no longer drips from the runnel. Transfer the absorbent to a glass trough lined with aluminium foil (free from rolling oil). Break up the magnesia with a clean spatula and spread out the absorbent on the aluminium foil in a layer about 1-2 cm thick. Dry at 160±1° for 24h. Pulverize the magnesia with mortar and pestle. Sieve the pulverized absorbent between 60-180 mesh. Use the magnesia retained on the 180-mesh sieve.
– Celite 545, Johns-Manvill Company, diatomaceous earth, or equivalent.
– Magnesium oxide-Celite 545 mixture (2+1) by weight: Place the magnesium oxide (60-180 mesh) and the Celite 545 in 2 to 1 proportions, respectively, by weight in a glass-stoppered flask large enough for adequate mixing. Shake vigorously for 10 min. Transfer the mixture to a glass trough lined with aluminium foil (free from rolling oil) and spread it out on a layer about 1 to 2 cm thick. Reheat the mixture at 160±10 for 2 h, and store in a tightly closed flask.
– Sodium sulfate, anhydrous, reagent grade, preferably in granular form: For each bottle of sodium sulfate reagent used, establish as follows the necessary sodium sulfate prewash to provide such filters required in the method: Place approximately 35 g of anhydrous sodium sulfate in a 30 ml coarse, fritted-glass funnel or in a 65 ml filter funnel with glass wool plug; wash with successive 15 ml portions of the indicated solvent until a 15 ml portion of the wash shows 0.00 absorbance per cm path length between 280 nm and 400 nm when tested as prescribed under “Organic solvents.” Usually three portions of wash solvent are sufficient.
Procedure
Before proceeding with the analysis of a sample, determine the absorbance in a 5 cm path cell between 250 nm and 400 nm for the reagent blank by carrying out the procedure, without a wax sample, at room temperature, recording the spectra after the extraction stage and after the complete procedure as prescribed. The absorbance per centimeter path length following the extraction stage should not exceed 0.040 in the wavelength range from 250 to 400 nm; the absorbance per cm path length following the complete procedure should not exceed 0.070 in the wavelength range from 250 to 299 nm, inclusive, nor 0.045 in the wavelength range from 300 nm to 400 nm. If in either spectrum the characteristic benzene peaks in the 250-260 nm region are present, remove the benzene by the procedure under “Organic solvents” and record absorbance again.
Place 300 ml of dimethyl sulfoxide in a 1-litre separatory funnel and add 75 ml of phosphoric acid. Mix the contents of the funnel and allow to stand for 10 min. (The reaction between the sulfoxide and the acid is exothermic. Release pressure after mixing, then keep runnel stoppered). Add 150 ml of isooctane and shake to pre-equilibrate the solvents. Draw off the individual layers and store in glass-stoppered flasks.
Place a representative 1-kg sample of wax, or if this amount is not available, the entire sample, in a beaker of a capacity about three times the volume of the sample and heat with occasional stirring on a steam bath until the wax is completely melted and homogenous. Weigh four 25 ± 0.2 g portions of the melted wax in separate 100 ml beakers. Reserve three of the portions for later replicate analyses as necessary. Pour one weighed portion immediately after remelting (on the steam bath) into a 500 ml separatory funnel containing 100 ml of the pre-equilibrated sulfoxide-phosphoric acid mixture that has been heated in the heating jacket at a temperature just high enough to keep the wax melted. (Note: In pre-heating the sulfoxide-acid mixture, remove the stopper of the separatory funnel at intervals to release the pressure).
Promptly complete the transfer of the sample to the funnel in the jacket with portions of the pre-equilibrated isooctane, warming the beaker, if necessary, and using a total volume of just 50 ml of the solvent. If the wax comes out of solution during these operations, let the stoppered funnel remain in the jacket until the wax redissolves. (Remove stopper from the funnel at intervals to release pressure).
When the wax is in solution, remove the funnel from the jacket and shake it vigorously for 2 min. Set up three 250-ml separatory funnels with each containing 30 ml of pre-equilibrated isooctane. After separation of the liquid phases, allow to cool until the main portion of the wax-isooctane solution begins to show a precipitate. Gently swirl the funnel when precipitation first occurs on the inside surface of the funnel to accelerate this process. Carefully draw off the lower layer, filter it slowly through a thin layer of glass wool fitted loosely in a filter runnel into the first 250-ml separatory funnel, and wash in tandem with the 30-ml portions of isooctane contained in the 250-ml separatory runnels. Shaking time for each wash is 1 min. Repeat the extraction operation with two additional portions of the sulfoxide-acid mixture, replacing the funnel in the jacket after each extraction to keep the wax in solution and washing each extractive in tandem through the same three portions of isooctane.
Collect the successive extracts (300 ml total) in a separatory funnel (preferably 2-litre), containing 480 ml of distilled water, mix, and allow to cool for a few minutes after the last extract has been added. Add 80 ml of isooctane to the solution and extract by shaking the funnel vigorously for 2 min. Draw off the lower aqueous layer into a second separatory funnel (preferably 2-litre) and repeat the extraction with 80 ml of isooctane. Draw off and discard the aqueous layer. Wash each of the 80-ml extracts three times with 100-ml portions of distilled water. Shaking time for each wash is 1 min. Discard the aqueous layers. Filter the first extract through anhydrous sodium sulfate pre-washed with isooctane (see Sodium sulfate under “Reagents and Materials” for preparation of filter) into a 250-ml Erlenmeyer flask (or optionally into the evaporation flask). Wash the first separatory funnel with the second 80-ml isooctane extract and pass through the sodium sulfate. Then wash the second and first separatory funnels successively with a 20-ml portion of isooctane and pass the solvent through the sodium sulfate into the flask. Add 1 ml of n-hexadecane and evaporate the isooctane on the steam bath under nitrogen. Discontinue evaporation when not over 1 ml of residue remains. To the residue, add a 10-ml portions of isooctane, reevaporate to 1 ml of hexadecane, and repeat this operation once more.
Quantitatively transfer the residue with isooctane to a 25-ml volumetric flask, make to volume, and mix. Determine the absorbance of the solution in the 5-cm path length cells compared to isooctane as reference between 280-400 nm (take care to lose none of the solution in filling the sample cell). Correct the absorbance values for any absorbance derived from reagents as determined by carrying out the procedure without a wax sample. If the corrected absorbance does not exceed the limits prescribed in the Characteristics, the wax meets the ultraviolet absorbance specifications. If the corrected absorbance per centimeter path length exceeds the limits prescribed in the Characteristics, proceed as follows:
Quantitatively transfer the isooctane solution to a 125-ml flask equipped with 24/40 joint and evaporate the isooctane on the steam bath under a stream of nitrogen to a volume of 1 ml of hexadecane. Add 10 ml of methyl alcohol and approximately 0.3 g of sodium borohydride (Minimize exposure of the borohydride to the atmosphere. A measuring dipper may be used). Immediately fit a water-cooled condenser equipped with a 24/40 joint and with a drying tube into the flask, mix until the borohydride is dissolved, and allow to stand for 30 min at room temperature, with intermittent swirling. At the end of this period, disconnect the flask and evaporate the methyl alcohol on the steam bath under nitrogen until the sodium borohydride begins to come out of the solution. Then add 10 ml of isooctane and evaporate to a volume of about 2-3 ml. Again, add 10 ml of isooctane and concentrate to a volume of approximately 5 ml. Swirl the flask repeatedly to assure adequate washing of the sodium borohydride residues.
Fit the tetrafluoroethylene polymer disc on the upper part of the stem of the chromatographic tube, then place the tube with the disc on the suction flask and apply the vaccum (approximately 135-mm Hg pressure). Weigh out 14 g of the 2+1 magnesium oxide-Celite 545 mixture and pour the adsorbent mixture into the chromatographic tube in approximately 3 cm layers. After the addition of each layer, level off the top of the adsorbent with a flat glass rod or metal plunger by pressing down firmly until the adsorbent is well packed. Loosen the topmost few ml of each adsorbent layer with the end of a metal rod before the addition of the next layer. Continue packing in this manner until all the 14 g of the adsorbent is added to the tube. Level off the top of the adsorbent by pressing down firmly with a flat glass rod or metal plunger to make the depth of the adsorbent bed approximately 12.5 cm in depth. Turn off the vacuum and remove the suction flask. Fit the 500-ml reservoir onto the top of the chromatographic column and pre-wet the column by passing 100 ml of isooctane through the column. Adjust the nitrogen pressure so that the rate of descent of the isooctane coming off of the column is between 2-3 ml per min. Discontinue pressure just before the last of the isooctane reaches the level of the adsorbent. (Caution: Do not allow the liquid level to recede below the adsorbent level at any time). Remove the reservoir and decant the 5 ml isooctane concentrate solution onto the column and with slight pressure again allow the liquid level to recede to barely above the adsorbent level. Rapidly complete the transfer similarly with two 5 ml portions of isooctane, swirling the flask repeatedly each time to assure adequate washing of the residue. Just before the final 5 ml wash reaches the top of the adsorbent, add 100 ml of isooctane to the reservoir and continue the percolation at the 2-3 ml per minute rate. Just before the last of the isooctane reaches the adsorbent level, add 100 ml of 10% benzene in isooctane to the reservoir and continue the percolation at the aforementioned rate. Just before the solvent mixture reaches adsorbent level, add 25 ml of 20% benzene in isooctane to the reservoir and continue the percolation at 2-3 ml per minute until all this solvent mixture has been removed from the column. Discard all the elution solvents collected up to this point. Add 300 ml of the acetone-benzene-water mixture to the reservoir and percolate through the column to elute the polynuclear compounds. Collect the eluate in a clean 1-litre separatory funnel. Allow the column to drain until most of the solvent mixture is removed. Wash the eluate three times with 300 ml portions of distilled water, shaking well for each wash. (The addition of small amounts of sodium chloride facilitates separation). Discard the aqueous layer after each wash. After the final separation, filter the residual benzene through anhydrous sodium sulfate pre-washed with benzene (see Sodium sulfate under “Reagents and Materials” for preparation of filter) into a 250-ml Erlenmeyer flask (or optionally into the evaporation flask). Wash the separatory funnel with two additional 20 ml portions of benzene which are also filtered through the sodium sulfate. Add 1 ml of n-hexadecane and completely remove the benzene by evaporation under nitrogen, using the special procedure to eliminate benzene as previously described under “Organic Solvents”. Quantitatively transfer the residue with isooctane to a 25-ml volumetric flask and adjust the volume. Determine the absorbance of the solution in the 5 cm path length cells compared to isooctane as reference between 250 – 400 nm. Correct for any absorbance derived from the reagents as determined by carrying out the procedure without a wax sample. If either spectrum shows the characteristic benzene peaks in the 250 – 260 nm region, evaporate the solution to remove benzene by the procedure under “Organic Solvents”. Dissolve the residue, transfer quantitatively, and adjust to volume in isooctane in a 25-ml volumetric flask. Record the absorbance again. If the corrected absorbance does not exceed the limits prescribed in the Characteristics the wax meets the ultraviolet absorbance specifications.