DNA Degradation of Genetically Modified Cottonseed Meal During Feed Processing

The effects of dry heating, wet heating, and extrusion on the degradation of DNA in cottonseed meal (CSM) were studied using polymerase chain reaction (PCR) and real-time PCR approach. Both the sad1 DNA, ranging between 128 and 883 bp in size, and the cry1Ab/c gene, ranging between 183 and 652 bp in size, were detectable in all dry-heated CSM and cottonseed. During wet heating, the sad1 gene (≥883 bp) and the cry1Ab/c (≥952 bp) gene were thoroughly degraded at 105 and 120 °C, respectively. Sizes from 128 to 530 bp for the sad1 gene and sizes from 183 to 652 bp for the cry1Ab/c gene were detected during extrusion at temperatures ranging from 75 to 135 °C. Fragments ≤883 bp for the sad1 gene and ≤952 bp for the cry1Ab/c gene were detected in all of the extruded samples with water content varying between 26 and 34 %. The copy number ratio of cry1Ab/c to sad1 in samples of Bt cottonseed meal decreased rapidly when the temperature increased during the heating process. In conclusion, feed processing markedly degrades the larger DNA fragments of sad1 and cry1Ab/c, with high temperature and water content being the main factors for that degradation.     

基准物的制备

有的药物研发实验室用色谱峰面积归一法表示药物主成分的含量,并据此优化合成条件．使用归一法的前提是试样中所有组分都以相同的响应因子被检测,否则,归一法的结果就与实际含量不一致．     

IUPAC Recommendations for Reference Standard Samples in pH Measurements

Consultations

IUPAC Recommendations for Reference Standard Samples in pH Measurements     

Consensus values for NIST biological and environmental Standard Reference Materials

The National Institute of Standards and Technology (NIST, formerly the National Bureau of Standards or NBS) has produced numerous Standard Reference Materials (SRM) for use in biological and environmental analytical chemistry. The value listed on the “NIST Certificate of Analysis” is the present best estimate of the “true” concentration of that element and is not expected to deviate from that concentration by more than the stated uncertainty. However, NIST does not certify the elemental concentration of every constituent and the number of elements reported in the NIST programs tends to be limited. Numerous analysts have published concentration data on these reference materials. Major journals in analytical chemistry, books, proceedings and “technical reports” have been surveyed to collect these available literature values. A standard statistical approach has been employed to evaluate the compiled data. Our methodology has been developed in a series of previous papers. Some subjective criteria are first used to reject aberrant data. Following these eliminations, an initial arithmetic mean and standard deviation (S.D.) are computed from remaining data for each element. All data now outside two S.D. from the initial mean are dropped and a second mean and S.D. recalculated. These final means and associated S.D. are reported as “consensus values” in our tables. Received: 25 April 1997 / Revised: 24 July 1977 / Accepted: 25 July 1997     

有机元素微量分析标准物质——茴香酸的研制

茴香酸的分子式为C_8H_8O_3,碳含量63.15%、氢含量5.30%、氧含量31.55%、甲氧基含量20.40%。该标样与日本元素分析恳谈会委员会、英国化学协会微量化学委员会所公布的微量化学标样之一——香草醛一样,都具有相同的碳、氢、氧和甲氧基含量,美国国家标准局(NBS)发行SRM142茴香酸作为微量分析中甲氧基的分析标样。     

关于水合离子标准生成焓的参比标准

针对学生因水合离子标准生成焓的参比标准而普遍产生的疑问 ,就教材表述的不确切处提出看法     

红景天甙和红景天甙元标准品的制备方法研究

用化学和高效液相制备色谱方法分离制备了红景天属植物提取物中甙及甙元的标准物，标准品纯度分别由１％～２％和１％提高到９９％和９７％以上。     

Determination of vitamins in food-matrix Standard Reference Materials

In recent years, the National Institute of Standards and Technology (NIST) has developed several food-matrix Standard Reference Materials (SRMs) characterized for vitamins and other organic nutrients. NIST uses several "modes" for assignment of analyte concentrations in SRMs, one of which includes the use of data provided by collaborating laboratories. Certification modes and liquid chromatographic methods that were used by NIST for value assignment of vitamin concentrations in recently introduced food-matrix SRMs are described in this paper. These materials and methods include vitamins D and E in coconut oil (SRM 1563) by gravimetry and multi-dimensional liquid chromatography (LC); vitamins A, E, and several B vitamins by reversed-phase LC and vitamin C by ion-exchange chromatography in infant formula (SRM 1846); and carotenoids and vitamins A and E by reversed-phase liquid chromatography in a baby food composite (SRM 2383).     

Developing qualitative LC-MS methods for characterization of Vaccinium berry Standard Reference Materials

Standard Reference Materials (SRMs) offer the scientific community a stable and homogenous source of material that holds countless application possibilities. Traditionally, the National Institute of Standards and Technology (NIST) has provided SRMs with associated quantitative information (certified values) for a select group of targeted analytes as measured in a solution or complex matrix. While the current needs of the SRM community are expanding to include non-quantitative data, NIST is attempting to broaden the scope of how and what information is offered to the SRM community by providing qualitative information about biomaterials, such as chromatographic fingerprints and profiles of untargeted identifications. In this work, metabolomic and proteomic profiling efforts were employed to characterize a suite of six Vaccinium berry SRMs. In the discovery phase, liquid chromatography-tandem mass spectrometry (LC-MS/MS) data was matched to mass spectral libraries; a subsequent validation phase based on multiple-reaction monitoring LC-MS/MS relied on both retention time matching of authentic standards along with fragmentation data for a qualitative overview of the most prominent organic compounds present. Definitive and putative identifications were determined for over 70 metabolites based on reporting guidelines set forth by the Metabolomics Standards Initiative (Metabolomics 3(3):211–221, 2007), and the capability of electrospray ionization mass spectrometry (ESI-MS) to profile untargeted metabolites within a complex matrix using mass spectral matching is demonstrated. Bottom-up proteomic analyses were possible using peptide databases translated from expressed sequence tags (ESTs). Homology searches provided identification of novel Vaccinium proteins based on homology to related genera. Chromatographic fingerprints of these berry materials were acquired for supplemental qualitative information to be provided to users of these SRMs. An unbounded set of qualitative data about a biomaterial is a valuable complement to quantitative information traditionally provided in NIST Certificates of Analysis.     

Production and certification of NIST Standard Reference Material 2372 Human DNA Quantitation Standard

Modern highly multiplexed short tandem repeat (STR) assays used by the forensic human-identity community require tight control of the initial amount of sample DNA amplified in the polymerase chain reaction (PCR) process. This, in turn, requires the ability to reproducibly measure the concentration of human DNA, [DNA], in a sample extract. Quantitative PCR (qPCR) techniques can determine the number of intact stretches of DNA of specified nucleotide sequence in an extremely small sample; however, these assays must be calibrated with DNA extracts of well-characterized and stable composition. By 2004, studies coordinated by or reported to the National Institute of Standards and Technology (NIST) indicated that a well-characterized, stable human DNA quantitation certified reference material (CRM) could help the forensic community reduce within- and among-laboratory quantitation variability. To ensure that the stability of such a quantitation standard can be monitored and that, if and when required, equivalent replacement materials can be prepared, a measurement of some stable quantity directly related to [DNA] is required. Using a long-established conventional relationship linking optical density (properly designated as decadic attenuance) at 260 nm with [DNA] in aqueous solution, NIST Standard Reference Material (SRM) 2372 Human DNA Quantitation Standard was issued in October 2007. This SRM consists of three quite different DNA extracts: a single-source male, a multiple-source female, and a mixture of male and female sources. All three SRM components have very similar optical densities, and thus very similar conventional [DNA]. The materials perform very similarly in several widely used gender-neutral assays, demonstrating that the combination of appropriate preparation methods and metrologically sound spectrophotometric measurements enables the preparation and certification of quantitation [DNA] standards that are both maintainable and of practical utility. Figure NIST Standard Reference Material (SRM) 2372 Human Quantitation Standard     

Preparation and analysis of a river sediment Standard Reference Material for the determination of trace organic constituents

Summary A river sediment Standard Reference Material (SRM) has been prepared and analyzed for determination of the concentrations of trace organic constituents. SRM 1939, Polychlorinated Biphenyls (PCBs) in River Sediment A, has been certified for the concentrations of three PCB congeners using the results obtained from capillary column gas chromatography with electron capture detection (GC-ECD) and from multidimensional (dual column) capillary gas chromatography with mass spectrometric detection (MCGC-MSD). For SRM certification, two independent analytical procedures are usually required. If only one analytical technique is used or if the procedures are not independent, then the concentrations are reported as noncertified or informational values rather than certified values. Noncertified values for 14 additional PCB congeners and five chlorinated pesticides, determined by GC-ECD, are also reported as well as noncertified concentrations for five polycyclic aromatic hydrocarbons (PAHs), determined using gas chromatography with mass spectrometric detection (GC-MSD). SRM 1939 complements SRM 1941, Organics in Marine Sediment, since both materials have 12 PCB congeners, five PAHs and five chlorinated pesticides in common. However, the concentrations differ by an order of magnitude for PAHs, and from one to over two orders of magnitude for the PCB congeners and chlorinated pesticides.     

Characterization of the NIST shellfish Standard Reference Material 4358

A new shellfish Standard Reference Material 4358 was developed by the National Institute of Standards and Technology through an international interlaboratory comparison that involved twelve laboratories-participants from nine countries. The results from the participants were statistically evaluated, and the most robust certified values were based on the median of laboratories’ reported means and the uncertainties derived using the bootstrap method. Massic activity certified values were established for fourteen radionuclides, five activity ratios, and informational massic activity values for eight more radionuclides and two activity ratios.     

国外标准参考物研制信息

美国国家标准与工艺研究所(NIST)以制作和供应标准参考物著称于世,现将该所研制参考物的动态报道如下。     

铅-钙合金光谱标样的制备与标定

通常用的铅 钙合金光谱标样比较缺乏 ,且钙含量范围一般只能做到 0 .2 %以下。本文试验此类合金光谱标样的制备与标定。可制备出钙含量范围从0 .0 1%～ 2 %的铅 钙合金标样 ,采用直读光谱分析法检验其均匀性 ,用原子吸收光谱法和ＥＤＴＡ容量法分析定值[1,2 ] ,制备出了结果满意的标准样品。1　试验部分1.1　主要仪器ＧＧＸ 5型原子吸收分光光度计 ,附钙空心阴极灯 (北京地质仪器厂 )。ＡＲＬ 4 4 6 0直读光谱仪 (瑞士ＡＲＬ公司 )ＧＷ 0 .15型中频感应炉1.2　试验方法利用中频感应炉、石墨坩埚 ,加金属铝作保护 ,将铅和钙于 (70 0± 30 )…     

臭氧标准参考光度计间接比对技术

参照国际计量局有关臭氧标准参考光度计(Standard Reference Photometer,SRP)间接比对的操作规程和美国环境保护署有关臭氧参考光度计之间比对验证的规定,采用臭氧传递标准,通过比对前的准备、比对过程的确定、比对结果的处理、比对指标的评价等步骤,开展了臭氧标准参考光度计间接比对实验。以SRPⅠ与SRPⅡ间接比对为例,SRPⅠ与SRPⅡ间接比对所得两个关系式的斜率分别为1.003 26和1.003 58,截距分别为0.109 05 nmol/mol和0.080 99 nmol/mol,结果显示两台SRP之间具有很好的一致性,比对结果符合美国环境保护署关于SRP之间比对的指标。建立了臭氧标准参考光度计之间的比对方法,适用于环境空气臭氧量值传递源头间的比对。     

Development and Certification of NIST Standard Reference Materials for Relative Raman Intensity Calibration

In analytical Raman spectroscopy it becomes increasingly important to employ a procedure for the correction of the relative intensity of Raman spectra. The determination of the intensity response function of a Raman instrument traditionally has been carried out through a white light source that has been calibrated for its relative spectral irradiance. While this method will furnish a correction curve to yield spectra corrected to relative Raman intensity, it is often cumbersome and fraught with experimental difficulties that can profoundly affect the reliability of the correction procedure. An alternate methodology that permits a simplified calibration of the Raman instrument response function is based on the use of luminescent glass standards that transfer a white light calibration onto the Raman measurement system. In this procedure, a measurement of the luminescence of an intensity standard, whose relative irradiance has been determined, provides a means to establish the instrument response function. Correction of measured spectra by this function furnishes spectra that are free of instrumental intensity artifacts. Based on this approach, NIST is developing a series of Standard Reference Materials (SRMs) for the calibration of Raman intensity. This process, and the results obtained thereby, is described for Raman spectroscopy measurements employing 785nm excitation. The procedure is valid for both macro-sampling and micro-sampling Raman work.     

EMMPRIN磷酸化突变质粒的构建及功能检测

利用聚合酶链式反应(PCR)定点诱变技术,对细胞外基质金属蛋白酶诱导因子(EMMPRIN)的2个磷酸化位点进行突变,构建了EMMPRIN磷酸化位点突变质粒.对其功能进行检测发现,EMMPRIN磷酸化位点突变质粒可在细胞内正常表达.研究结果显示,突变质粒可抑制肿瘤细胞的增殖(P<0.05),表明EMMPRIN可能与肿瘤细胞的增殖相关.     

Determination of non-ortho polychlorinated biphenyls in environmental Standard Reference Materials

The concentrations of three non-ortho ("coplanar") polychlorinated biphenyls, 3,3',4,4'-tetrachlorobiphenyl (IUPAC PCB 77), 3,3',4,4',5-pentachlorobiphenyl (IUPAC PCB 126), and 3,3',4,4',5,5'-hexachlorobiphenyl (IUPAC PCB 169), were determined in five NIST Standard Reference Materials (SRMs) of environmental and biological interest. The measured levels were approximately between (0.2 to 1.3) ng/g in SRM 1588a (Organics in Cod Liver Oil), (0.3 to 9) ng/g in SRM 1944 (New York/New Jersey Waterway Sediment), (0.2 to 0.4) ng/g in SRM 1945 (Organics in Whale Blubber), (1 to 18) ng/g in SRM 2974 (Organics in Freeze-dried Mussel Tissue [Mytilus edulis]), and (0.1 to 0.4) ng/g in candidate SRM 1946 (Lake Superior Fish Tissue). PCB 169 was present at < 0.1 ng/g in SRMs 1944 and 2974.