Development of clenbuterol reference materials: lyophilized bovine eye samples free of clenbuterol (CRM 673) and containing clenbuterol (CRM 674)

The certification by inter-laboratory testing of two candidate reference materials (RMs) for the mass concentration of the anabolic agent clenbuterol in bovine eye material is described: RM 674 with ca 10 microg clenbuterol per kg of eye matrix and RM 673 clenbuterol-free eye matrix as the negative control (<0.50 microg kg(-1)). Both candidate RMs were certified by eleven EU laboratories, and sixty-six accepted replicate measurements were included in the "Certification Study". The precision of the measurement process was assessed by calculation of the standard variation determined within each laboratory during the certification step. The study was performed according to the "Guidelines for the production and certification of BCR reference materials" and to "ISO guide 31, 33, and 35". The certified clenbuterol mass concentration for clenbuterol-free eye material CRM 673 (calculated on the basis of clenbuterol as the free base) was <0.50 microg kg(-1). The corresponding concentration for clenbuterol-containing eye material CRM 674 was 9.42 +/- 0.88 microg kg(-1). These certified values are very close to the desired target concentration of <0.5 microg kg(-1) and ca 10 microg kg(-1). This study has demonstrated that successful certification of clenbuterol-containing and clenbuterol-free bovine eye materials is possible.     

Certification of the methylmercury content in SRM 2977 mussel tissue (organic contaminants and trace elements) and SRM 1566b oyster tissue

The methylmercury content in two new marine bivalve mollusk tissue Standard Reference Materials (SRMs) has been certified using results of analyses from the National Institute of Standards and Technology (NIST) and two other laboratories. The certified concentrations of methylmercury were established based on the results from four and six different (independent) analytical methods, respectively, for SRM 1566b Oyster Tissue (13.2 +/- 0.7 microg/kg) and SRM 2977 Mussel Tissue (organic contaminants and trace elements) (36.2 +/- 1.7 microg/kg). The certified concentration of methylmercury in SRM 1566b is among the lowest in any certified reference material (CRM).     

Development of reference materials for paralytic shellfish poisoning toxins

A project was undertaken to develop mussel reference materials that were certified for their mass fractions of saxitoxin and decarbamoyl-saxitoxin. Fifteen laboratories from various European countries participated. Three of these had major responsibility for substantial parts of the work and overall coordination of the project. The project involved 4 main activities: (1) procurement and characterization of calibrants; (2) improvement of analytical methodology; (3) preparation of reference materials, including homogeneity and stability studies; (4) 2 interlaboratory studies and a certification exercise. The joint activities resulted in 3 homogeneous and stable reference materials: 2 lyophilized mussel materials with and without naturally incurred paralytic shellfish poisoning (PSP) toxins, and a saxitoxin enrichment solution. The reference materials were certified with respect to their saxitoxin and decarbamoyl-saxitoxin content. The lyophilized mussel material with PSP toxins (CRM 542) contained <0.07 mg saxitoxin x 2HCl/kg and 1.59 +/- 0.20 mg decarbamoyl-saxitoxin x 2HCl/kg. The lyophilized mussel material without PSP toxins (CRM 543) contained <0.07 mg saxitoxin x 2HCl/kg and <0.04 mg decarbamoyl-saxitoxin x 2HCl/kg. The certified value of the saxitoxin mass fraction in the saxitoxin enrichment solution (CRM 663) was 9.8 +/- 1.2 microg/g.     

Determination of methylmercury in fish using focused microwave digestion following by Cu2+ addition, sodium tetrapropylborate derivatization, n-heptane extraction, and gas chromatography-mass spectrometry

The analytical procedure for analysis of methylmercury in fish was developed. It involves microwave-assisted digestion with alkaline solution (tetramethylammonium hydroxide), addition of Cu2+, aqueous-phase derivatization of methylmercury with sodium tetrapropylborate, and subsequent extraction with n-heptane. The methylmercury derivative was desorbed in the splitless injection port of a gas chromatograph and subsequently analyzed by electron impact mass spectrometry. Optimum conditions allowed sample throughout to be controlled by the instrumental analysis time (near 7 min per sample) but not by the sample preparation step. At the power of 15-30, 45, and 60-75 W, sample preparation time is only 3.5, 2.5, and 1.5 min, respectively. The proposed method was finally validated by the analysis of three biological certified reference materials, BCR CRM 464 tuna fish, NRC DORM-2 dogfish muscle, and NRC DOLT-2 dogfish liver. The detection limit of the overall procedure was found to be 40 ng/g of biological tissue for methylmercury. The recovery of methylmercury was 91.2-95.3% for tuna, 89.3-94.7% for marlin, and 91.7-94.8% for shark, respectively. The detected and certified values of methylmercury of three biological certified reference materials were as follows: 5.34 +/- 0.30 microg/g (mean +/- S.D.) and 5.50 +/- 0.17 microg/g for CRM 464 tuna fish, 4.34 +/- 0.24 and 4.47 +/- 0.32 microg/g for NRC DORM-2 dogfish muscle, and 0.652 +/- 0.053 and 0.693 +/- 0.055 microg/g for NRC DOLT-2 dogfish liver, respectively. It indicated that the method was well available to quantify the methylmercury in fish.     

Development and certification of a coal fly ash certified reference material for selected polycyclic aromatic hydrocarbons

The development and certification of a coal fly ash certified reference material (CRM) for polycyclic aromatic hydrocarbons (PAH) is described; this is the first natural matrix CRM for organic environmental analysis in China. The homogeneity and stability of this material have been tested by HPLC. The concentrations of several PAH were determined by use of two independent, different methods--solvent extraction-HPLC analysis with UV detection coupled with fluorescence detection (FLD) and solvent extraction, isolation with a silica column, and GC analysis with flame ionization detection (FID). Five certified values were determined: phenanthrene 7.1 +/- 2.6 microg g(-1), anthracene 2.0 +/- 0.8 microg g(-1), fluoranthene 7.4 +/- 1.9 microg g(-1), pyrene 7 +/- 2 microg g(-1), and benzo[a]pyrene 1.3 +/- 0.3 microg g(-1). Reference values for several other PAH are also suggested.     

Determination of phosphorus in small amounts of protein samples by ICP–MS

Inductively coupled plasma mass spectrometry (ICP-MS) is used for phosphorus determination in protein samples. A small amount of solid protein sample (down to 1 micro g) or digest (1-10 micro L) protein solution was denatured in nitric acid and hydrogen peroxide by closed-microvessel microwave digestion. Phosphorus determination was performed with an optimized analytical method using a double-focusing sector field inductively coupled plasma mass spectrometer (ICP-SFMS) and quadrupole-based ICP-MS (ICP-QMS). For quality control of phosphorus determination a certified reference material (CRM), single cell proteins (BCR 273) with a high phosphorus content of 26.8+/-0.4 mg g(-1), was analyzed. For studies on phosphorus determination in proteins while reducing the sample amount as low as possible the homogeneity of CRM BCR 273 was investigated. Relative standard deviation and measurement accuracy in ICP-QMS was within 2%, 3.5%, 11% and 12% when using CRM BCR 273 sample weights of 40 mg, 5 mg, 1 mg and 0.3 mg, respectively. The lowest possible sample weight for an accurate phosphorus analysis in protein samples by ICP-MS is discussed. The analytical method developed was applied for the analysis of homogeneous protein samples in very low amounts [1-100 micro g of solid protein sample, e.g. beta-casein or down to 1 micro L of protein or digest in solution (e.g., tau protein)]. A further reduction of the diluted protein solution volume was achieved by the application of flow injection in ICP-SFMS, which is discussed with reference to real protein digests after protein separation using 2D gel electrophoresis.The detection limits for phosphorus in biological samples were determined by ICP-SFMS down to the ng g(-1) level. The present work discusses the figure of merit for the determination of phosphorus in a small amount of protein sample with ICP-SFMS in comparison to ICP-QMS.     

Determination of arsenic in scalp hair samples from exposed subjects using microwave-assisted digestion with and without enrichment based on cloud point extraction by electrothermal atomic absorption spectrometry

A simple and rapid cloud point extraction (CPE) procedure was applied for preconcentration of trace quantities of arsenic (As) in scalp hair samples. The samples were subjected to microwave-assisted digestion in a mixture of nitric acid and hydrogen peroxide (2 + 1, v/v) prior to preconcentration by CPE. The As in digested samples was complexed with ammonium pyrrolidine dithiocarbamate (APDC), and the resultant As-PDC complex was extracted by a nonionic surfactant, octylphenoxypolyethoxyethanol (Triton X-114). After centrifugation, the surfactant-rich phase was diluted with 0.1 M HNO3 in methanol and analyzed by electrothermal atomic absorption spectrometry. The experimental parameters, i.e., amount of APDC, concentration of Triton X-114, equilibrium temperature and time, were optimized. For validation of the proposed method, a certified reference material (CRM) of human hair (BCR 397) was used. No significant difference (P > 0.05) was observed between the experimental results and certified values of the CRM (paired t-test). The LOD and LOQ obtained under the optimal conditions were 0.025 and 0.083 microg/kg, respectively. The developed method was applied for the determination of As in scalp hair samples from male and female subjects of two villages of Khairpur Mir's, Pakistan.     

Species-specific isotope dilution analysis of mono-, di,and tri-butyltin compounds in sediment using gas chromatography-inductively coupled plasma mass spectrometry with synthesized 118Sn-enriched butyltins

A species-specific isotope dilution (ID) method is described for the determination of mono-, di, and tri-butyltin compounds in sediment by gas chromatography-inductively coupled plasma mass spectrometry (GC-ICP-MS), where the mixture of 118Sn-enriched butyltin compounds synthesized in our laboratory was used as a spike. A correction method for the mass bias, a quantitative extraction of the butyltins from sediment, and an assay for the concentration of the standard solution for the reverse ID procedure were investigated to achieve a reliable ID analysis. The spike solution was added with tri-propyltin (TPrT), and the butyltins were extracted by mechanical shaking into acetic acid-tropolone-toluene. The extracted butyltins were ethylated with sodium tetraethylborate and measured by GC-ICP-MS. The mass bias correction factor for the butyltins was calculated with the measured area ratio of 120Sn/118Sn of TPrT in each chromatographic run, and the correction was carried out. The mass bias was well corrected with this in-run correction (the standard uncertainties of the corrected 120Sn/118Sn for the butyltins were in the range 0.03-0.45%, typically 0.25%, with triplicate measurement corresponding to 0.02-0.37% mass bias). The extraction efficiency of mono-butyltin (MBT) from sediment was improved by using tropolone-toluene as the solvent. Well-defined standard solutions for the reverse-ID procedure could be obtained by an assay for the purities of the natural abundance butyltin chloride reagents used for preparing the standard solutions. Overall uncertainties associated with the present method were estimated, where the sediment certified reference materials, PACS-2 and BCR 646, were analyzed. The uncertainty arising from the extraction was the main contributor to the overall uncertainties for MBT and di-butyltin (DBT) determinations, while with the case of tri-butyltin (TBT) determination the uncertainties arising from the purity of TBT chloride reagent used for preparing the standard solution was a large contributor to the overall uncertainties although the uncertainty arising from the extraction was also a main contributor. The analytical results of MBT, DBT, and TBT in both reference materials, except for MBT results in PACS-2, were in good agreement with the certified values in each. The result of MBT in PACS-2 (0.677 +/- 0.049 microg g(-1) as tin, mean +/- expanded uncertainty) was significantly higher than the certified value (0.45 +/- 0.05 microg g(-1)), but closely matched with the lately reported values (Rajendran, Tao, Nakazato and Miyazaki, Analyst, 2000, 125, 1757: 0.62 +/- 0.02 microg g(-1); Chiron, Roy, Cottier and Jeannot, J. Chromatogr. A, 2000, 879, 137: 0.634 +/- 0.082 microg g(-1); Alonso, Encinar, Gonzalez and Sanz-Medal, Anal. Bioanal. Chem., 2002, 373, 432: 0.64 +/- 0.04 microg g(-1). The present method is concluded to be reliable for the determination of MBT, DBT, and TBT in sediment.     

Micro-heterogeneity study of trace elements in BCR CRM 680 by means of synchrotron micro-XRF

BCR CRM 680 is a newly released reference material (RM) with a polyolefinic matrix, doped with various metallic compounds in trace concentrations, to be used for calibration of multi-element trace analytical methods. The micro-heterogeneity of this new CRM was investigated to evaluate the suitability as a RM for trace-level micro analytical techniques. Synchrotron micro-XRF, a trace-level micro analytical method, allows to quantitatively measure the degree of heterogeneity of inorganic trace constituents in solid materials with a homogeneous matrix. The procedure for calculating the minimal sampling mass for homogeneous measurements was employed for BCR CRM 680. By repeating the entire procedure on several samples of the same material, the repeatability of the micro-heterogeneity characterization based on micro-XRF was investigated. Afterwards, the micro-heterogeneity results from the BCR CRM 680 material were used to evaluate the suitability of the micro-heterogeneity procedure by means of a Monte Carlo simulation model. Also the existence of nuggets in the polymer material is looked into.     

Micro-heterogeneity study of trace elements in BCR CRM 680 by means of synchrotron micro-XRF

BCR CRM 680 is a newly released reference material (RM) with a polyolefinic matrix, doped with various metallic compounds in trace concentrations, to be used for calibration of multi-element trace analytical methods. The micro-heterogeneity of this new CRM was investigated to evaluate the suitability as a RM for trace-level micro analytical techniques. Synchrotron μ-XRF, a trace-level micro analytical method, allows to quantitatively measure the degree of heterogeneity of inorganic trace constituents in solid materials with a homogeneous matrix. The procedure for calculating the minimal sampling mass for homogeneous measurements was employed for BCR CRM 680. By repeating the entire procedure on several samples of the same material, the repeatability of the micro-heterogeneity characterization based on μ-XRF was investigated. Afterwards, the micro-heterogeneity results from the BCR CRM 680 material were used to evaluate the suitability of the micro-heterogeneity procedure by means of a Monte Carlo simulation model. Also the existence of nuggets in the polymer material is looked into.     

A multielement masking method using magnesium hydroxide coprecipitation for the selective determination of lead in water samples by differential pulse anodic stripping voltammetry.

We present a new multielement masking method using magnesium hydroxide coprecipitation for the selective determination of Pb by differential pulse anodic stripping voltammetry (DPASV). The recovery of Pb in the masking method was over 95%, while interfering ions (Cd(2+), Co(2+), Cu(2+), Fe(3+), Mn(2+), and Ni(2+)) could be removed at 100% from the analytical sample. A linear regression was obtained in the Pb concentration from 10 to 1000 microg kg(-1) in the existence of 100 microg kg(-1) of the interfering ions. When this method was applied to the determination of Pb in a natural water-standard reference material (NIST 1640), the determined value for Pb in this work (25.4 +/- 4.1 microg kg(-1)) almost agreed with the certified value (27.89 +/- 0.14 microg kg(-1)).     

Highly sensitive determination of iodide by ion chromatography with amperometric detection at a silver-based carbon paste electrode

A silver-based solid carbon paste electrode was developed for use as a detector in ion chromatography (IC) for the sensitive determination of iodide in real samples. Micro- and nano-particles of silver were investigated for the fabrication of different electrodes. The iodide assay was based on IC with amperometric detection (IC-AD) at a silver composite electrode polarized at +0.080 V versus Ag/AgCl. Free iodide and organoiodide compounds were studied. The detection process was characterized by studying the redox behavior of iodide ions at both silver and silver composite electrodes by cyclic voltammetry (CV). The presence of iodide ions in solution was found to considerably facilitate metallic silver oxidation, with response currents directly related to iodide concentration. The calibration curve at the selected silver carbon paste electrode was linear in the concentration range comprised between 0.635 microg/L and 63.5 microg/L iodide. The relative standard deviation (R.S.D.) for successive injections was below 3% for all iodide standard solutions investigated. The limit of detection (LOD) was 0.47 microg/L (3.7 nmol/L) for an injection volume of 20 microL, i.e. 74 fmol injected. The IC-AD method was successfully applied to the determination of iodide in complex real samples such as table salts, sea products and iodide bound drug compounds. The analytical accuracy was verified by the assay of iodide in milk powder from an iodide certified reference material (CRM) Community Bureau of Reference (BCR) 150.     

毛细管电泳-电感耦合等离子体质谱联用测定海藻中铅形态化合物

建立了毛细管电泳( CE)与电感耦合等离子体质谱( ICP-MS)联用技术测定铅离子( PbⅡ)、三甲基铅(TML)和三乙基铅(TEL)3种不同形态铅化合物的方法,以及海藻中不同形态铅化合物的提取技术,实现了海藻中3种铅形态化合物的定性定量分析。结果表明：以70 mmol/L H3BO3-17.5 mmol/L Na2B4O7(pH 8.90)为缓冲溶液,在最佳CE-ICP-MS条件下3种铅化合物20 min内可实现有效分离,重现性较好,迁移时间RSD﹤4%,峰面积的RSD﹤5%;在10~200μg/L 范围内3种铅化合物线性较好,相关系数大于0.90; PbⅡ、TML和TEL的CE-ICP-MS检出限(3S/N,以Pb计)分别为0.091,0.023和0.030μg/L;采用分步提取海藻中Pb元素,提取率高达80%以上,以藻体为基底 PbⅡ, TML 和 TEL 回收率分别为103.6%,95.7%和90.6%;通过检测紫菜和海带中铅含量,结果显示藻体内Pb主要以PbⅡ形式存在。本方法具有简单、高效、样品消耗量少等优点,可为海藻及其它海产品的质量控制提供技术支撑。     

Isotope dilution determination of polycyclic aromatic hydrocarbons in olive pomace oil by gas chromatography-mass spectrometry

A gas chromatographic (GC) method with mass spectrometry detection (MS) for the determination of eight polycyclic aromatic hydrocarbons (PAHs) in olive pomace oil has been developed. The oil was diluted with n-pentane and extracted by liquid-liquid partition with dimethyl sulphoxide (DMSO). After water addition and back-extraction with cyclohexane, a thin-layer chromatography on silica gel was performed as a further purification step. The PAHs spot was scraped off from the plate and the final extract was concentrated and analysed by GC-MS in full scan mode. The eight PAHs under investigation were determined in the presence of the corresponding labelled compounds added as internal standards to the sample at the beginning of the analytical process. The identified PAHs were then quantified by the isotope dilution methodology assuring the compensation of the concentration of each analyte for any variation in the sample preparation. The method precision was satisfactory with relative standard deviation (R.S.D.) values in the range 3.6-12.7% for all PAHs. The average recovery rates ranged from 69.0 to 97.5%. Accuracy was also calculated for benzo[k]fluoranthene, benzo[a]pyrene, indeno[1,2,3-cd]pyrene and benzo[ghi]perylene by analysing a certified reference material (CRM 458, coconut oil) with adequate results. All response curves exhibited a linear fit from 0.1 to 10 microg ml(-1) and the determination coefficients R2 were better than 0.9942. The limits of detection (0.1-0.4 microg kg(-1)) were acceptable when compared with the maximum permitted limit of 2 microg kg(-1) for each of the eight considered PAHs and 5 microg kg(-1) for the sum of the eight PAHs established by the Italian legislation. Measurement uncertainty was finally calculated identifying and quantifying the uncertainty components of the analytical process. The relative expanded uncertainties (Uc), expressed as percent values were in the range 8.5-11.4% thus appropriate for residues quantification in the range of concentrations considered in the present study.     

Determination of selenium in marine biological tissues by transverse heated electrothermal atomic absorption spectrometry with longitudinal Zeeman background correction and automated ultrasonic slurry sampling.

A fast, sensitive, and reliable method for determination of selenium in marine biological tissues by electrothermal atomic absorption spectrometry with slurry sampling was developed. Slurries were prepared from fresh and frozen seafood samples that were previously homogenized, dried, and ground; particle sizes <100 microm were taken for analysis. A 3% (v/v) HNO3 solution containing 0.01% (v/v) Triton X-100 was used as slurry diluent. Slurries were mixed on an automated ultrasonic slurry sampler at 20% amplitude for 30 s just before an aliquot was injected into the furnace. The method was successfully validated against the following certified reference materials: NRCC CRM DORM-2 (Dogfish muscle); NRCC CRM TORT-2 (Lobster hepatopancreas); NRCC CRM DOLT-2 (Dogfish liver); and BCR CRM 278 (Mussel tissue), and was subsequently applied to determination of Se in 10 marine biological samples. The influences of the drying procedure (oven-, microwave-, and freeze-drying), matrix modifier amount, mass of solid material in cup, and pipetting sequence are discussed. The limit of determination of Se was 0.16 microg/g and the repeatability, estimated as between-batch precision, was in the range of 4-8%. Se contents in the samples ranged from 0.6 to 2.8 microg/g. The proposed method should be useful for fast assessment of the daily dietary intake of Se.     

INAA and PIXE for the determination of the contents of extractable sediment

The three-stage BCR sequential step reference extraction procedure was applied to the reference material BCR CRM 601, especially developed for fractionation studies. Extracted fractions were analyzed for Cr, Ni, Zn, Cd, and Pb, by k ₀-standardized instrumental neutron activation (k ₀ INAA) and proton induced X-ray emission (PIXE), and flame atomic absorption spectrometry (FAAS). Sample preparation procedures were developed for both k ₀ INAA and PIXE techniques, related to the evaporation of the solutions in order to get solid samples for neutron and proton irradiation. Quality control was assessed by intercomparison of the analytical results obtained by the applied techniques, which included results for a few certified reference materials. In the extracted fractions, chromium concentration was not determined accurately by both nuclear techniques. Concerning Cd, Ni, Pb, and Zn, the results were in general in good agreement with the certified values and FAAS. Some incomplete separation of the residue might have occurred.     

Comparison of methods used for the preparation of biological CRM's

The starting material for two certified and one candidate reference material was obtained from dried grass specially cultivated on a selected and well prepared soil. The Community Bureau of Reference (BCR) of the Commission of the European Communities produced two certified reference materials (CRM's) from this dried grass: a rye grass material (CRM 281) certified in 1988 for the quality control of trace and toxic element analyses and a hay powder material (CRM 129) certified in 1989 for monitoring trace and minor elements. A fraction of the dried grass was used in 1993 for the preparation of a hay powder with a particle size of <63 m using newly developed grinding techniques.This paper compares the production methods of these three materials and the obtained particle size distribution of the powders. The analytical evaluation of these production methods was carried out by solid sampling Zeeman atomic absorption spectrometry for the determination of Cd, Pb and Zn.     

Certification of the methylmercury content in SRM 2977 Mussel Tissue (organic contaminants and trace elements) and SRM 1566b Oyster Tissue

The methylmercury content in two new marine bivalve mollusk tissue Standard Reference Materials (SRMs) has been certified using results of analyses from the National Institute of Standards and Technology (NIST) and two other laboratories. The certified concentrations of methylmercury were established based on the results from four and six different (independent) analytical methods, respectively, for SRM 1566b Oyster Tissue (13.2 ± 0.7 μg/kg) and SRM 2977 Mussel Tissue (organic contaminants and trace elements) (36.2 ± 1.7 μg/kg). The certified concentration of methylmercury in SRM 1566b is among the lowest in any certified reference material (CRM).     

Speciation of arsenic in mussels by the coupled system liquid chromatography-UV irradiation-hydride generation-inductively coupled plasma mass spectrometry

A method has been developed for the determination of seven arsenic species in mussel tissues by liquid chromatography-hydride generation-UV photo-oxidation and detection by inductively coupled plasma mass spectrometry. In order to determine the different species, two ion-exchange columns (anionic and cationic) were used with phosphate and nitric acid/ammonium nitrate as mobile phases, respectively. The optimisation of the conditions for separation, photo-oxidation and hydride generation is described. For each of these species, the limits of detection and repeatability are reported with the entire system coupling. This system was applied to the analysis of certified reference material (CRM 278) and mussels collected from Barcelona harbour. Extractions were achieved in methanol/water (1:1) using low-power focused microwaves as leaching process. As expected, arsenobetaine was the main compound extracted from both materials; the typical concentrations found were between 1 and 7 mg kg(-1). Other organoarsenical compounds, probably arsenosugars, were extracted in a concentration range of 0.3-1.5 mg kg(-1) in both cases. Amounts of dimethylarsinate (DMA) were found to be significant in the CRM 278, but very low in mussels from Barcelona harbour. The low limits of detection of the coupled system allow us to quantify low contents of other species (As(V), arsenocholine and monomethylarsonate (MMA)).     

Certification of the mass fractions of Ca,Cu, Cl,I, Fe,K, Mg,P, Pb,N, Na and Zn in skim milk powder

Analyses of milk and milk products are routinely performed by a number of dairy laboratories to control the quality of these products with regard to e.g. nutritional components and potential exposure to toxic elements. In order to improve and control the quality of such analyses the Community Bureau of Reference (BCR) has organized series of certification campaigns to produce reference material of milk certified for a variety of elements and compounds. The increasing demand is such that the stock of some of these materials is now exhausted. Consequently, the BCR decided to produce a new batch of CRM of skim milk powder certified for its contents of Ca, Cu, Cl, I, Fe, K, Mg, P, Pb, N, Na and Zn (CRM 063R). This material was carefully prepared (spray-drying) and its homogeneity and long term stability was verified. This paper presents the certification work performed.