Rolf Zeisler

Involvement of TLR2 and TLR4 in inflammatory immune responses induced by fine and coarse ambient air particulate matter

Induction of proinflammatory mediators by alveolar macrophages exposed to ambient air particulate matter has been suggested to be a key factor in the pathogenesis of inflammatory and allergic diseases in the lungs. However, receptors and mechanisms underlying these responses have not been fully elucidated. In this study, we examined whether TLR2, TLR4, and the key adaptor protein, MyD88, mediate the expression of proinflammatory cytokines and chemokines by mouse peritoneal macrophages exposed to fine and coarse PM. TLR2 deficiency blunted macrophage TNF‐α and IL‐6 expression in response to fine (PM2.5), while not affecting cytokine‐inducing ability of coarse NIST Standard Reference Material (SRM 1648) particles. In contrast, TLR4−/− macrophages showed inhibited cytokine expression upon stimulation with NIST SRM 1648 but exhibited normal responses to PM2.5. Preincubation with polymyxin B markedly suppressed the capacity of NIST SRM 1648 to elicit TNF‐α and IL‐6, indicating endotoxin as a principal inducer of cytokine responses. Overexpression of TLR2 in TLR2/4‐deficient human embryonic kidney 293 cells imparted PM2.5 sensitivity, as judged by IL‐8 gene expression, whereas NIST SRM 1648, but not PM2.5 elicited IL‐8 expression in 293/TLR4/MD‐2 transfectants. Engagement of TLR4 by NIST SRM 1648 induced MyD88‐independent expression of the chemokine RANTES, while TLR2‐reactive NIST IRM PM2.5 failed to up‐regulate this response. Consistent with the shared use of MyD88 by TLR2 and TLR4, cytokine responses of MyD88−/− macrophages to both types of air PM were significantly reduced. These data indicate differential utilization of TLR2 and TLR4 but shared use of MyD88 by fine and coarse air pollution particles.

Preparation of a mixed human diet material for the determination of nutrient elements, selected toxic elements and organic nutrients: A preliminary report

Using 201 foods from the United States Food and Drug Administrations Total Diet Study (FDA TDS), a mixed diet composite (USDIET-I) was prepared to represent the intake of 25-30-year-old males in the United States. Proximate analyses, phytate determination, and assays for nutrient elements and selected toxic elements, as well as organic nutrients were carried out on this composite. As part of a quality control exercise for a coordinated research program, atomic absorption spectrophotometry, inductively coupled atomic emission spectrometry, colorimetry and neutron activation analysis were used to determine up to 30 elements in this diet material. A comparison of the daily intakes of As, Ca, Cd, Cu, Fe, Hg, K, Mg, Mn, Na, P, Se and Zn from the composite USDIET-I shows excellent to good agreement with FDA TDS values calculated from results of single food analyses. These USDIET-I results demonstrate the feasibility of the mixed diet concept as a viable approach for a reliable assessment of daily intakes, especially for a number of elements such as Cd, Cr, Hg and Mo that occur at low concentrations in individual food products. Simultaneously, stability of some organic nutrients during storage was also investigated. Initial findings suggest that this program may also be useful in the development of reference materials for organic nutrients, for which there is a great need. These aspects are discussed.

Determination of inorganic constituents in marine mammal tissues

Analyses of selected tissues from the Alaska Marine Mammal Tissue Archival Project (AMMTAP) have provided comprehensive information related to levels of 36 trace elements and methyl-mercury in marine mammal tissues. Liver, kidney and muscle tissues from two northern fur seals, four ringed seals and six belukha whales were analyzed. The bulk of the investigated tissues and additional tissues from a total of 65 marine mammals are banked in the AMMTAP. The results are compared to literature values for trace element concentrations in marine mammal tissues and their relevance to environmental studies is discussed.

Ultratrace determination of platinum in biological materials via neutron activation and radiochemical separation

A neutron activation analysis scheme based upon a radiochemical separation of the activation products has been developed. The method utilizes the inherent sensitivity of the activation reaction198Pt(n, γ)199Pt and counting of the daughter nuclide199Au. This nuclide is radiochemically separated from interfering activities by homogeneous precipitation as elemental gold. The remaining interference of the secondary reaction197Au(n,γ)198 Au(n,γ)199Au from gold in the samples is quantitatively assessed and corrected. During this process accurate gold concentrations in the samples are obtained at ultratrace levels. The analysis scheme is applied to gold and platinum determinations in biological Standard Reference Materials and human liver specimens. Gold and platinum are determined at concentrations of 5·10−11 g/g, and at higher levels.

Trace elements in human livers using quality control in the complete analytical process

The validity and intercomparability of data in research related to medical, environmental, and geochemical health problems is of utmost concern and requires specific consideration in the development of an analytical approach. The Environmental Protection Agency/National Bureau of Standards Pilot Environmental Specimen Bank Program provides a vehicle for developing the precise and accurate determination of trace constituents in human livers. This approach, when implemented, gives specific consideration to a valid relationship between the analytical result and the true value in the sample. This is accomplished by minimizing contamination of the sample and/or loss of constituents, and by assuring representative analytical test portions. The analysis of the liver specimens is performed under strict quality control. The applied analytical techniques (atomic absorption spectrometry, isotope dilution mass spectrometry, neutron activation analysis, and voltammetry) have been verified for accuracy through the analysis of Standard Reference Materials. In addition, several elements are determined using two or three of these independent techniques. The first year of the program provided results on 31 elements including Se and Pb in 36 human livers.

Activation analysis opportunities using cold neutron beams

Guided beams of cold neutrons being installed at a number of research reactors may become increasingly available for analytical research. A guided cold beam will provide higher neutron fluence rates and lower background interferences than in present facilities. In an optimized facility, fluence rates of 109 n·cm−2·s−1 are obtainable. Focusing a large area beam onto a small target will further increase the neutron intensity. In addition, the shift to lower neutron energy increases the effective cross sections. The absence of fast neutrons and gamma rays permits detectors to be placed near the sample without intolerable background, and thus the efficiency for counting prompt gamma rays can be much higher than in present systems. Measurements made at the hydrogen cold source of the FRJ-2 (DIDO) reactor at the KFA provide a numerical evaluation of the improvements in PGAA with respect to signal-to-background ratios of important elements and matrices.

Neutron captue prompt gamma-ray activation analysis at the NIST Cold Neutron Research Facility

An instrument for neutron capture prompt gamma-ray activation analysis (PGAA) has been constructed as part of the Cold Neutron Research Facility at the 20 MW National Institute of Standards and Technology Research Reactor. The neutron fluence rate (thermal equivalent) is 1.5·108 n ·cm−2·s−1, with negligible fast neutrons and gamma-rays. With compact geometry and hydrogen-free construction, the sensitivity is sevenfold better than an existing thermal instrument. Hydrogen background is thirtyfold lower.

Sample preparation protocols for realization of reproducible characterization of single-wall carbon nanotubes

Harmonized sample pre-treatment is an essential first step in ensuring quality of measurements as regards repeatability, interlaboratory reproducibility and commutability. The development of standard preparation methods for single-wall carbon nanotube (SWCNT) samples is therefore essential to progress in their investigation and eventual commercialization. Here, descriptions of sample preparation and pre-treatment for the physicochemical characterization of SWCNTs are provided. Analytical methods of these protocols include scanning electron microscopy (dry, wet), transmission electron microscopy (dry, wet), atomic force microscopy, inductively coupled plasma mass spectrometry, neutron activation analysis, Raman spectroscopy (dry, wet), UV–Vis–NIR absorption and photoluminescence spectroscopy, manometric isothermal gas adsorption and thermogravimetric analysis. Although sample preparation refers to these specific methods, application to other methods for measurement and characterization of SWCNTs can be envisioned.

Biological Specimen Banking in Arctic Research: An Alaska Perspective

The cryogenic archival of biological specimens for retrospective analysis is of significant value for present and future research on population genetics, pathology, systematics, toxicology and environmental monitoring. This realization is emphasized by the increasing support of this activity by various government agencies, institutions and international groups. The international Arctic community is no exception. Canada has been conducting such activities in association with environmental monitoring programs for many years. Similar efforts appear to be underway in other polar nations. From the perspective of the United States Arctic, the Alaska Marine Mammal Tissue Archival Project (AMMTAP) was the earliest organized effort to develop an environmental specimen bank specifically designed for longterm archival of biological specimens under cryogenic conditions. The AMMTAP emphasizes use of standardized rigorous sampling and archival protocols, procedures that minimize contamination of samples during collection and maintaining a detailed record of sample history. The development of this specimen bank, recent activities of this project and other cryogenic specimen banks being developed in Alaska are described.

A RADIOCHEMICAL PROCEDURE FOR ULTRATRACE DETERMINATION OF CHROMIUM IN BIOLOGICAL MATERIALS

Chromium is one of the most difficult elements to accurately determine at the naturally occuring, ultratrace levels normally found in uncontaminated biological samples. In view of the importance of Cr, both as an essential and as a toxic element, efforts have focused on developing a simple, yet reliable, radiochemical procedure for Cr determination using neutron activation analysis. A number of problem areas have been identified in earlier methods, and an improved radiochemical separation procedure, based upon the liquid/liquid extraction of Cr(VI) into a solution of tribenzylamine/chloroform, has been developed. The fast neutron interference from Fe has been evaluated for the highly thermal RT-4 facility of the NBS Research Reactor, and Cr concentrations have been determined in samples of whole human blood collected under clean conditions and in two certified reference materials.