Ultrafine particles cross cellular membranes by nonphagocytic mechanisms in lungs and in cultured cells.High concentrations of airborne particles have been associated with increased pulmonary and cardiovascular mortality, with indications of a specific toxicologic role for ultrafine particles (UFPs; particles < 0.1 [micro]). Within hours after the respiratory system is exposed to UFPs, the UFPs may appear in many compartments of the body, including the liver, heart, and nervous system. To date, the mechanisms by which UFPs penetrate boundary membranes and the distribution of UFPs within tissue compartments of their primary and secondary target organs are largely unknown. We combined different experimental approaches to study the distribution of UFPs in lungs and their uptake by cells. In the in vivo experiments, rats inhaled an ultrafine titanium dioxide aerosol of 22 nm count median diameter. The intrapulmonary distribution of particles was analyzed 1 hr or 24 hr after the end of exposure, using energy-filtering transmission electron microscopy “TEM” redirects here. For other uses, see TEM (disambiguation). Transmission electron microscopy (TEM) is an imaging technique whereby a beam of electrons is transmitted through a specimen, then an image is formed, magnified and directed to appear either for elemental microanalysis microanalysis /mi·cro·anal·y·sis/ (-ah-nal´i-sis) the chemical analysis of minute quantities of material. microanalysis the chemical analysis of minute quantities of material. of individual particles. In an in vitro study, we exposed pulmonary macrophages Macrophages White blood cells whose job is to destroy invading microorganisms. Listeria monocytogenes avoids being killed and can multiply within the macrophage. and red blood cells Red blood cells Cells that carry hemoglobin (the molecule that transports oxygen) and help remove wastes from tissues throughout the body. Mentioned in: Bone Marrow Transplantation red blood cells to fluorescent polystyrene microspheres (1, 0.2, and 0.078 [micro]m) and assessed particle uptake by confocal laser scanning microscopy Confocal laser scanning microscopy (CLSM or LSCM) is a technique for obtaining high-resolution optical images.[1] The key feature of confocal microscopy is its ability to produce in-focus images of thick specimens, a process known as . Inhaled ultrafine titanium dioxide particles were found on the luminal side of airways and alveoli Alveoli Small air sacs or cavities in the lung that give the tissue a honeycomb appearance and expand its surface area for the exchange of oxygen and carbon dioxide. , in all major lung tissue compartments and cells, and within capillaries. Particle uptake in vitro into cells did not occur by any of the expected endocytic processes, but rather by diffusion or adhesive interactions. Particles within cells are not membrane bound and hence have direct access to intracellular proteins, organelles, and DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. , which may greatly enhance their toxic potential. Key words: aerosol, erythrocytes Erythrocytes Red blood cells. Mentioned in: Bartonellosis erythrocytes (ē·rithˑ·rō·sīts), n.pl red blood cells. , lungs, macrophages, microscopy, nanoparticles, rats, surfactant Surfactant Definition Surfactant is a complex naturally occurring substance made of six lipids (fats) and four proteins that is produced in the lungs. It can also be manufactured synthetically. . ********** High concentrations of airborne particles have been associated with increased pulmonary and cardiovascular mortality, with indications of a specific toxicologic role for ultrafine particles (UFPs; particles with diameters < 0.1 [micro]m) (Peters et al. 1997). UFPs may induce inflammatory and prothrombotic responses, promoting atherosclerosis, thrombogenesis, and the occurrence of other cardiovascular events (Schulz et al. 2005). Human data suggest that inhaled UFPs influence lung physiology (Pietropaoli et al. 2004). UPFs may also affect the autonomic nervous system autonomic nervous system: see nervous system. autonomic nervous system Part of the nervous system that is not under conscious control and that regulates the internal organs. It includes the sympathetic, parasympathetic, and enteric nervous systems. or act directly on cells in various organs and induce mutations (Harder et al. 2005; Samet et al. 2004). After exposure of the respiratory system to UFPs, the UFPs may appear within hours in many compartments of the body, including the liver, heart, and nervous system (Brown et al. 2002; Kreyling et al. 2002; Oberdorster et al. 2004). UFPs are formed by gas-to-particle conversion or by incomplete fuel combustion. Despite considerable efforts to reduce air pollution, the environmental burden by UFPs may have increased rather than decreased over time (Kreyling et al. 2003). Moreover, the fast-growing nanotechnology industry generates new UFPs daily, which may become aerosolized Adj. 1. aerosolized - in the form of ultramicroscopic solid or liquid particles dispersed or suspended in air or gas aerosolised gaseous - existing as or having characteristics of a gas; "steam is water is the gaseous state" at some stage and may present additional health risks. UFPs possess increased toxicity compared with larger particles composed of the same materials (Ferin et al. 1992). Their environmental burden is characterized by high number concentrations but low mass concentrations. Thus, a relatively large surface area per unit mass facilitates adsorption of various organic compounds from the ambient air and enhances interaction with biological molecules within the organism. Deposition of UFPs in the respiratory system is caused by diffusional displacement. Depending on particle size, deposition occurs efficiently in the nose, the conducting airways, and the alveoli. Although particles with diameters > l [micro]m usually remain on the epithelial surface upon their deposition (Gehr et al. 1990; Geiser et al. 2003; Schurch et al. 1990) and are subjected to clearance by cough, mucociliary transport, and/or phagocytosis phagocytosis: see endocytosis. Phagocytosis A mechanism by which single cells of the animal kingdom, such as smaller protozoa, engulf and carry particles into the cytoplasm. by macrophages, UFPs seem to penetrate the boundary membranes of the lungs rapidly--a unique feature for insoluble particles (Brown et al. 2002; Kreyling et al. 2002; Oberdorster et al. 2002). In addition, transport across the olfactory epithelium and accumulation in the brain were reported for various UFP UFP United Federation of Planets (Star Trek) UFP Union des Forces Progressistes (French: Union of the Forces Progressists, Quebec provincial party) UFP URL Filtering Protocol types (Oberdorster 2004). In vitro experiments revealed penetration of UFPs into mitochondria of macrophages and epithelial cells that was associated with oxidative stress and mitochondrial mitochondrial pertaining to mitochondria. mitochondrial RNAs a unique set of tRNAs, mRNAs, rRNAs, transcribed from mitochondrial DNA by a mitochondrial-specific RNA polymerase, that account for about 4% of the total cell RNA that damage (Li et al. 2003). Because everyone on earth inevitably inhales thousands to millions of UFPs with each breath, it is important to assess health risks by UFP air pollution. The costs of actions to be taken to reduce ambient aerosol particles are high and will affect the economy greatly, presenting an urgent need to clarify the fate of inhaled UFPs. To date, the mechanisms by which UFPs penetrate boundary membranes and the distribution of UFPs within tissue compartments of their primary and secondary target organs are largely unknown. This study is the first to investigate the distribution of inhaled UFPs within lungs at the individual particle level and combines different experimental approaches--an in vivo inhalation study in rats and an in vitro cell exposure study on pulmonary macrophages and red blood cells (RBCs). In the in vivo experiments, rats inhaled an ultrafine titanium dioxide aerosol of 22 nm count median diameter (CMD CMD cerebromacular degeneration. ) during 1 hr, resulting in a deposition of 4-5 [micro]g Ti[O.sub.2] per animal. The intrapulmonary distribution of deposited particles was analyzed immediately or 24 hr after the end of exposure, using energy-filtering transmission electron microscopy (EFTEM EFTEM Energy-Filtering Transmission Electron Microscopy ) to allow elemental microanalysis of individual particles (Kapp et al. 2004). In the in vitro study, we exposed cultured porcine pulmonary macrophages and human RBCs to fluorescent polystyrene microspheres with diameters of 1, 0.2, and 0.078 [micro]m and assessed particle uptake by confocal laser scanning microscopy (CLSM CLSM Confocal Laser Scanning Microscope CLSM Controlled Low-Strength Material CLSM Conical Log Spiral Mobile CLSM Committee of Lunacy and Surreal Madness (band) ). Materials and Methods Animals. The animal experiments were conducted under federal guidelines for the use and care of laboratory animals (German Animal Protection Law) and were approved by the District of Upper Bavaria (Approval No. 211-2531-108/99) and by the GSF GSF Gross Square Feet (architectural design and construction) GSF Genoa Social Forum (umbrella anti-G8 group) GSF GameSpy Forums GSF Government Superannuation Fund (New Zealand) Institutional Animal Care and Use Committee Institutional Animal Care and Use Committees are of central importance to the application of laws to animal research in the United States. Most research involving laboratory animals is funded by the United States National Institutes of Health or other federal agencies. , as well as in accordance with the Swiss Federal Act on Animal Protection and the Swiss Animal Protection Ordinance. Ten young, adult, male WKY/NCrl BR rats [body weight (bw) 250 [+ or -] 10 g (mean [+ or -] SD; Charles River, Sulzfeld, Germany] were housed under standard conditions, with access to food and water ad libitum, in a room controlled for humidity (55% relative humidity) and temperature (22[degrees]C) and with lighting on a 12-hr day/night cycle. Animals were anesthetized a·nes·the·tize also a·naes·the·tize tr.v. a·nes·the·tized, a·nes·the·tiz·ing, a·nes·the·tiz·es To induce anesthesia in. a·nes by intramuscular injection of a mixture of medetomidine (Domitor; 150 [micro]g/100 g bw; Pfizer GmbH, Karlsruhe, Germany), midazolam (Dormicum; 0.2 mg/100 g bw; Hoffmann-La Roche AG, Grenzach-Wyhlen, Germany), and Fentanyl fentanyl /fen·ta·nyl/ (fen´tah-nil) an opioid analgesic; the citrate salt is used as an adjunct to anesthesia, in the induction and maintenance of anesthesia, in combination with droperidol (or similar agent) as a neuroleptanalgesic, and (0.5 [micro]g/100 g bw; Janssen-Cilag GmbH, Neuss, Germany) for inhalation and lung fixation and anticoagulated by intraperitoneal injection of 2,000 IU heparin (Heparin-Natrium-ratiopharm, ratiopharm GmbH, Ulm/Donautal, Germany) for lung fixation (Kapp et al. 2004). Anesthesia was antagonized by subcutaneous injection of atipamezole (Antisedan; Pfizer GmbH), flumazenil (Anexate, Hoffmann-La Roche AG), and naloxone naloxone /nal·ox·one/ (nal-ok´son) an opioid antagonist, used as the hydrochloride salt in opioid toxicity, opioid-induced respiratory depression, and hypotension associated with septic shock. (Narcanti, Janssen Animal Health, Neuss, Germany). Aerosols and inhalation. Titanium is suitable for EFTEM because it does not interfere with the heavy metals used for tissue preparation (Kapp et al. 2004). Ti[O.sub.2] is inert and nonpathogenic (Templeton 1994), and ultrafine aerosols thereof remain as insoluble particles (Donaldson et al. 2002). Generally, commercially available Ti[O.sub.2] particles (Degussa, Dusseldorf, Germany) show a positive Zeta potential of 20-30 mV as measured by Malvern Zetasizer 3000 HS (Malvern Instruments Ltd., Malvern, Worcestershire, UK) The generation and inhalation of the Ti[O.sub.2] aerosol used in this study has been described in detail by Kapp et al. (2004). Briefly, ultrafine Ti[O.sub.2] aerosols were generated with a Palas spark generator (Palas GmbH, Karlsruhe, Germany) in a pure argon plus 0.1% oxygen stream. The aerosol was quasi-neutralized by a radioactive [sup.85]Kr source, diluted, and conditioned for inhalation. Particle size distribution The particle size distribution[1] ("PSD") of a powder, or granular material, or particles dispersed in fluid, is a list of values or a mathematical function that defines the relative amounts of particles present, sorted according to size. and number concentration were monitored continuously by a differential electrical mobility particle sizer and a condensation particle counter. An aerosol of 22 nm CMD (geometric SD of 1.7) was produced. The mean number concentration was 7.3 x [10.sup.6] particles/[cm.sup.3] (SD 0.5 x [10.sup.6] particles/[cm.sup.3]), corresponding to a mass concentration of 0.11 mg/[m.sup.3]. The 22 nm particles measured as aerosol particles are already agglomerates of smaller primary structures formed immediately after spark ignition and condensation. The estimated size of the primary structures was 4 nm as derived from the measured specific surface area of 330 [m.sup.2]/g of the UFPs produced in this study and the Ti[O.sub.2] bulk density of 4.2 g/[cm.sup.3]. Each anesthetized rat was placed in an airtight plethysmograph plethysmograph /ple·thys·mo·graph/ (ple-thiz´mo-grah) an instrument for recording variations in volume of an organ, part, or limb. ple·thys·mo·graph n. box. The animals inhaled the aerosol in pairs (one each for the 1-hr and 24-hr examinations) for 1 hr via an endotracheal tube by negative-pressure ventilation (-1.5 Pa) at a breathing frequency of 45/min, resulting in a minute volume of about 200 [cm.sup.3]/min (Kreyling et al. 2002). From breathing and aerosol parameters, the deposited amount of Ti[O.sub.2] was calculated to be 4-5 [micro]g in each rat. After aerosol exposure, anesthesia of one of the paired rats was antagonized as described above, and the animal was returned to its cage for 24 hr. Lung fixation and tissue preparation. Lungs were fixed either 1 hr or 24 hr after the aerosol inhalation by sequential intravascular intravascular /in·tra·vas·cu·lar/ (in?trah-vas´ku-lar) within a vessel. in·tra·vas·cu·lar adj. Within one or more blood vessels. perfusion with buffered 2.5% glutaraldehyde glutaraldehyde /glu·ta·ral·de·hyde/ (gloo?tah-ral´de-hid) a disinfectant used in aqueous solution for sterilization of non-heat–resistant equipment; also used as a tissue fixative for light and electron microscopy. (Agar Agar, in the Bible Agar (ā`gər), the same as Hagar. agar, substance obtained from seaweed agar (ä`gär, ā`–, ăg`är) Scientific Ltd., Piano GmbH, Wetzlar, Germany), 1.0% osmium tetroxide (Simec, Zofingen, Switzerland), and 0.5% uranyl acetate (Fluka Chemie GmbH, Sigma-Aldrich, Buchs, Switzerland). Lungs were then subjected to systematic tissue sampling, dehydration in a graded series of ethanol, and embedding in Epon (Fluka) (Im Hof et al. 1989; Kapp et al. 2004). Ultrathin ul·tra·thin adj. Very thin. ([less than or equal to] 50 nm) sections were cut from five to eight tissue blocks per animal, mounted onto uncoated 600-mesh copper grids, and stained with uranyl acetate and lead citrate citrate /cit·rate/ (sit´rat) a salt of citric acid. citrate phosphate dextrose (CPD) anticoagulant citrate phosphate dextrose solution. (Ultrostain, Leica, Glattbrugg, Switzerland). Particle localization Customizing software and documentation for a particular country. It includes the translation of menus and messages into the native spoken language as well as changes in the user interface to accommodate different alphabets and culture. See internationalization and l10n. and elemental microanalysis in situ. On ultrathin sections, 12 fields, corresponding to an area of 1,820 [micro][m.sup.2] each, were systematically subsampled and investigated for the presence and localization of Ti[O.sub.2] particles in a LEO 912 transmission electron microscope (LEO, Oberkochen, Germany) equipped with an in-column energy filter allowing energy dispersion for element specific contrast. Ti[O.sub.2] particles were identified by parallel electron energy-loss spectroscopy (parallel-EELS), electron spectroscopic spec·tro·scope n. An instrument for producing and observing spectra. spec  tro·scop imaging, and image-EELS (Kapp et al. 2004). For elemental microanalysis, we used the [L.sub.2,3] edge of Ti at 456 eV energy loss. We obtained bright-field and structure-sensitive micrographs (recorded at 250 eV), as well as element-specific contrast for Ti[O.sub.2], by digital acquisition. Cell culture experiments. Porcine lung macrophages (provided by K. McCullough and H. Gerber, Institute for Virus Diseases and Immune Prophylaxis, Mittelhausern, Switzerland) were cultured at [10.sup.6] cells/mL in two-chamber slides (VWR International AG, Dietikon, Switzerland) for 24 hr at 37[degrees]C and 5% C[O.sub.2] in RPMI RPMI Rapid Prototyping & Manufacturing Institute RPMI Roswell Park Memorial Institute RPMI Royal Park Memorial Institute (culture medium) 1640 medium (containing 25 mM Hepes; LabForce AG, Nunningen, Switzerland) with 10% fetal bovine serum Fetal bovine serum ( or foetal bovine serum) is serum taken from the fetuses of cows. Fetal Bovine Serum (or FBS) is the most widely used serum in the culturing of cells. In some papers the expression foetal calf serum is used. (LabForce), 1% L-glutamine (LabForce), and 1% penicillin/streptomycin (Gibco BRL BRL In currencies, this is the abbreviation for the Brazilian Real. Notes: The currency market, also known as the Foreign Exchange market, is the largest financial market in the world, with a daily average volume of over US $1 trillion. , Invitrogen AG, Basel, Switzerland). Human RBCs, always freshly isolated from the same donor, were cultured at 8 x [10.sup.6] cells/mL and for 6-24 hr, as described above. For CLSM, fluorescent polystyrene microspheres with diameters of 1, 0.2, and 0.078 [micro]m (Fluoresbrite plain yellow green; Polysciences, Chemie Brunschwig AG, Basel, Switzerland) were added to the cells at [10.sup.10] particles/mL in supplement-free RPMI 1640 medium for 4 hr. To inhibit phagocytic phag·o·cyt·ic adj. 1. Of or relating to phagocytes. 2. Of, relating to, or characterized by phagocytosis. phagocytic emanating from or pertaining to phagocytes. uptake, cells were pretreated with cytochalasin D (cytD, 10 [micro]g/mL; Fluka) for 30 min and during incubation with particles (Thiele et al. 2001). Macrophages were then washed in phosphate-buffered saline (PBS PBS in full Public Broadcasting Service Private, nonprofit U.S. corporation of public television stations. PBS provides its member stations, which are supported by public funds and private contributions rather than by commercials, with educational, cultural, ), fixed in 3% paraformaldehyde/PBS, treated with 0.1 M glycine/PBS, permeabilized with 0.2% Triton X-100/PBS, and stained for F-actin with rhodamine-phalloidin (1:100; Molecular Probes, VWR International AG, Lucerne Lucerne (l  sûrn`), Ger. Luzern (ltsĕrn`), canton (1993 pop. , Switzerland) for 60 min at 37[degrees]C. RBCs were fixed in 2.5% glutaraldehyde/PBS, resulting in a red autofluorescence. Preparations were mounted in PBS:glycerol glycerol, glycerin, glycerine, or 1,2,3-propanetriol (prō`pāntrī'ŏl), CH2OHCHOHCH2OH, colorless, odorless, sweet-tasting, syrupy liquid. (2:1) containing 170 mg/mL Mowiol 4-88 (Calbiochem, VWR International AG). For TEM TEM 1. transmission electron microscope. 2. triethylenemelamine. 3. transmissible encephalopathy of mink. analysis, RBCs were incubated with 0.025 [micro]m gold particles (ANAWA ANAWA Anti-Nuclear Alliance of Western Australia Trading SA, Wangen, Switzerland) at 6.6 x [10.sup.10] particles/mL. RBCs were fixed with buffered 2.5% glutaraldehyde, 1% osmium tetroxide, and 0.5% uranyl acetate, and prepared for TEM as described above for lung tissue. Microscopic analysis of cultured cells. We used a MicroRadiance system from Bio-Rad (Hemel Hempstead, UK) combined with an inverted inverted reverse in position, direction or order. inverted L block a pattern of local filtration anesthesia commonly used in laparotomy in the ox. Nikon microscope (Eclipse TE3000; lasers: GHe/Ne 543 nm and Ar 488 nm) (Nikon, Kusnacht, Switzerland). Optical sections with a voxel dimension of 50 x 50 x 200 nm were taken with a 100x/1.4 plan-apochromate objective. We performed image processing and visualization using IMARIS software (Bitplane AG, Zurich, Switzerland). We applied a deconvolution In mathematics, deconvolution is an algorithm-based process used to reverse the effects of convolution on recorded data.[1] The concept of deconvolution is widely used in the techniques of signal processing and image processing. algorithm using Huygens2 software (Scientific Volume Imaging B.V., Hilversum, Netherlands) to increase axial and lateral resolutions and to decrease noise (Rothen-Rutishauser et al. 1998). Experiments were performed in triplicate or quadruplicate quad·ru·pli·cate adj. 1. Multiplied by four; quadruple. 2. Fourth in a group of four identical things. n. One of a group of four identical things. tr. & intr.v. , and 30-50 cells were scanned by CLSM for each data point. We examined ultrathin sections of RBCs incubated with gold particles in a Philips 300 TEM at 60 kV (Philips, Zurich, Switzerland). Results Distribution of inhaled UFPs in lungs. We found Ti[O.sub.2] particles on the luminal side of airways and alveoli as well as within each tissue compartment of the lung (Figures 1 and 2). Particles were localized within epithelial and endothelial cells, within fibroblasts Fibroblasts A type of cell found in connective tissue; produces collagen. Mentioned in: Skin Grafting and between collagen fibrils in the connective tissue, within blood capillaries, and even within RBCs (Figure 1). Intracellular particles were localized most often in the cytoplasm and rarely within the nucleus. Particles within cells were not membrane bound. On average, 79.3 [+ or -] 7.6% (mean [+ or -] SD) of the particles were found on the luminal side of airways and alveoli, 4.6 [+ or -] 2.5% were within epithelial or endothelial cells, 4.8 [+ or -] 4.5% within the connective tissue, and 11.3 [+ or -] 3.9% within the capillaries. The relative distributions of particles among different lung compartments at 1 hr and at 24 hr after inhalation were not different from each other and correlated with the volume fractions of the respective compartments (Figure 2). [FIGURES 1-2 OMITTED] Uptake of UFPs by macrophages and RBCs. We studied the uptake of fine (1-0.2 [micro]m) and ultrafine (< 0.1 [micro]m) fluorescent microspheres in cultured macrophages as a model for phagocytic cells and in human RBCs as a model for nonphagocytic cells. Additionally, we treated macrophage macrophage /mac·ro·phage/ (mak´ro-faj) any of the large, mononuclear, highly phagocytic cells derived from monocytes that occur in the walls of blood vessels (adventitial cells) and in loose connective tissue (histiocytes, phagocytic cultures with cytD to block phagocytosis. Cells were prepared for CLSM, and a deconvolution algorithm was applied to increase lateral as well as axial resolution. We found particles of all sizes within macrophages (Figure 3A), however, with different percentages of cells involved in particle uptake. On average, 77 [+ or -] 15% (mean [+ or -] SD) of the macrophages contained UFPs, 21 [+ or -] 11% contained 0.2 [micro]m particles, and 56 [+ or -] 30% contained 1 [micro]m particles (Figure 3B). CytD did not inhibit the uptake of ultrafine and 0.2 [micro]m particles but blocked the uptake of 1 [micro]m particles by these cells (Figure 3B). We found ultrafine and 0.2 [micro]m, but not 1 [micro]m, particles in RBCs (Figure 4A). TEM analysis of RBCs incubated with 0.025 [micro]m gold particles showed that intracellular particles were not membrane bound (Figure 4B). [FIGURES 3-4 OMITTED] Discussion The ultrastructural analyses of lung tissue demonstrated that I hr after aerosol inhalation, 24% of ultrafine Ti[O.sub.2] particles, on average, were located within and beyond the epithelial barrier (i.e., in the main lung tissue compartments, in the cytoplasm, and in the nucleus of the cells). These results confirm data from human studies, where the inhalation of ultrafine carbon particles affected pulmonary diffusing capacity (Pietropaoli et al. 2004), suggesting that particles in the interstitium have physiologic effects. This study also provides evidence for some particle translocation translocation /trans·lo·ca·tion/ (trans?lo-ka´shun) the attachment of a fragment of one chromosome to a nonhomologous chromosome. Abbreviated t. into the microvasculature microvasculature /mi·cro·vas·cu·la·ture/ (-vas´kul-ah-cher) the finer vessels of the body, as the arterioles, capillaries, and venules. . In previous studies on iridium iridium (ĭrĭd`ēəm), metallic chemical element; symbol Ir; at. no. 77; at. wt. 192.22; m.p. about 2,410°C;; b.p. about 4,130°C;; sp. gr. 22.55 at 20°C;; valence +3 or +4. particles, we found minute fractions of particles translocated into secondary target organs (Kreyling et al. 2002; Semmler et al. 2004b). Different particle materials--iridium versus Ti[O.sub.2]--may have resulted in different particle translocation patterns, and we do not know the exact composition and structure of the ultrafine particle surface, which is likely to influence particle translocation. The present study focuses on particle distribution within the primary target organ, the lung, and the results do not determine which fraction of particles may have escaped the lung microvasculature to be systemically circulated. Particles found within cells were not membrane bound, indicating a nonendocytic uptake. In addition, the overall distribution pattern of the particles in the lungs (i.e., the percentages of particles in the different lung compartments) at 1 hr and at 24 hr after particle inhalation was the same and was correlated with the volume densities of the corresponding lung compartments, implying that ultrafine Ti[O.sub.2] particles can move between tissue compartments without restraint. Our results are in contrast with those obtained by Stearns et al. (2001), who studied the uptake of ultrafine Ti[O.sub.2] particles in vitro in the A549 epithelial cell line. They found that membrane-bound vesicles contained mostly large aggregates of Ti[O.sub.2]. Sometimes vesicles with clusters consisting of as few as two to three particle profiles were observed. In a pilot study in vitro with porcine macrophages, we obtained similar results (data not shown). Whether these clusters contained few particles only or were sectioned through the top of larger ones is not known. However, because ultrafine Ti[O.sub.2] aggregate very quickly in polar liquids such as cell culture medium and because particle concentration was fairly high, as seen from micrographs, it is very likely that particles aggregated within the cell culture medium and that cells engulfed these large clusters by an endocytic pathway. Particle agglomeration ag·glom·er·a·tion n. 1. The act or process of gathering into a mass. 2. A confused or jumbled mass: on the lung epithelium during the 1-hr inhalation, however, is very unlikely because of the size of the inner lung surface and the number of deposited UFPs. The fact that 80% of the retained Ti[O.sub.2] particles were still on the luminal side of the epithelium even 24 hr after inhalation is surprising and in contrast to previous studies on the lavageability of ultrafine iridium particles, where only 20% of the particles could be lavaged from the epithelial surfaces 24 hr after inhalation (Kreyling et al. 2002). The low lavageability of ultrafine iridium particles in contrast to high lavageability of 80% of 0.5-10-[micro]m particles (Oberdorster et al. 2002) was interpreted as either higher adhesion of UFPs to epithelial membranes or epithelial uptake and penetration of UFPs into the interstitium. The large fraction of Ti[O.sub.2] particles on the luminal side of the epithelium in the present study strongly supports higher adhesion of UFPs to epithelial structures. However, it must also be considered that proteins are very likely to bind rapidly to the particles, which then may affect the further metabolic fate of the particles in terms of their adhesion, residence time on the epithelium or uptake, and even penetration through the epithelium. Along this line, the difference of the two particle materials and surfaces may have led to binding of those proteins, which then may have mediated major uptake and penetration of iridium particles into and through the epithelium. We already have first evidence that ultrafine commercial Ti[O.sub.2] particles bind more readily to other proteins in the lung-lining fluid than carbonaceous car·bo·na·ceous adj. Consisting of, containing, relating to, or yielding carbon. carbonaceous Adjective of, resembling, or containing carbon Adj. 1. and amorphous silica particles (Semmler et al. 2004a). Microscopic analyses of phagocytic and nonphagocytic cells incubated with different particle types showed that macrophages take up fine and uhrafine polystyrene microspheres and that treatment with cytD inhibits the uptake of 1.0-[micro]m particles, but not uptake of the smaller particles, by these cells. Ultrafine polystyrene and gold particles also entered RBCs and were not membrane bound. The mechanisms of intracellular uptake of macromolecules Macromolecules A large molecule composed of thousands of atoms. Mentioned in: Gene Therapy macromolecules , particles, and even cells are subsumed as endocytosis endocytosis (ĕn'dōsītō`səs), in biology, process by which substances are taken into the cell. When the cell membrane comes into contact with a suitable food, a portion of the cell cytoplasm surges forward to meet and surround . Material to be ingested is progressively enclosed by the plasma membrane, which eventually detaches to form an endocytic vesicle vesicle /ves·i·cle/ (ves´i-k'l) 1. a small bladder or sac containing liquid. 2. a small circumscribed elevation of the epidermis containing a serous fluid; a small blister. . Phagocytosis and pinocytosis pinocytosis: see endocytosis. are distinguished by the size of endocytic vesicles formed. Phagocytosis, a receptor-mediated, actin-based process, is characteristic for neutrophils neutrophils (ner·ō·trōˑ·filz), n.pl white blood cells with cytoplasmic granules that consume harmful bacteria, fungi, and other foreign materials. , macrophages, and dendritic cells. It is the main mechanism for the clearance of insoluble 1- to 3-[micro]m particles from the alveoli. Pinocytosis involves the ingestion ingestion /in·ges·tion/ (-chun) the taking of food, drugs, etc., into the body by mouth. in·ges·tion n. 1. The act of taking food and drink into the body by the mouth. 2. of fluid and solutes via vesicles of about 100 nm in diameter. There are at least four basic mechanisms, most of which can be demonstrated in lungs and involve specific receptor-ligand interactions: a) macropinocytosis, b) clathrin-mediated, actin-based endocytosis, c) caveolae-mediated endo- or transcytosis, and d) clathrin- and caveolae-independent endocytosis (Conner and Schmid 2003). Kruth et al. (1999) described an additional endocytic process, patocytosis, in which hydrophobic polystyrene particles < 0.5 [micro]m are transported through induced plasma membrane channels into an extensive labyrinth of interconnected membrane-bound compartments. None of these endocytic pathways, all of which include vesicle formation, is likely to account for the translocation of UFPs in our study, as intracellularly localized particles were not membrane bound. Moreover, because RBCs contained UFPs and cytD treatment of macrophages did not prevent UFP translocation into these cells, particle uptake by any actin-based mechanism can also be excluded. Transport via pores, as suggested for lung-blood substance exchange (Conhaim et al. 1988; Hermans and Bernard 1999), is another potential mechanism for UFP translocation. Ti[O.sub.2] particles may diffuse through such pores. A transport mechanism by diffusion is consistent with the observed spatial distribution of UFPs in our inhalation study. Thus far, signal-mediated transport via pores has been demonstrated only for ultrafine gold particles of up to 39 nm in diameter, through the nuclear pore complex in Xenopus oocytes, where transport velocities depended on particle size (Pante and Kann 2002). Passive uptake (not triggered by receptor-ligand interactions) may also occur by electrostatic, Van der Waals, or steric steric /ste·ric/ (ster´ik) pertaining to the arrangement of atoms in space; pertaining to stereochemistry. ster·ic or ster·i·cal n. interactions, subsumed under "adhesive interactions" (Rimai et al. 2000). Rimai et al. showed that 8-[micro]m glass particles were approximately 90% engulfed by a polystyrene substrate, compared with 22-pro particles, which were only 30% engulfed. However, the influence of particle size on their engulfment was not clarified in these publications. Several concepts for the nonspecific nonspecific /non·spe·cif·ic/ (non?spi-sif´ik) 1. not due to any single known cause. 2. not directed against a particular agent, but rather having a general effect. nonspecific 1. engulfment of particles through interfacial structures (including cell membranes) have been suggested. A thermodynamic ther·mo·dy·nam·ic adj. 1. Characteristic of or resulting from the conversion of heat into other forms of energy. 2. Of or relating to thermodynamics. model using the "wettability criterion" was successful in predicting passive particle uptake, although it did not take into account the elastic properties of the cell membrane (Chen et al. 1997). In another thermodynamic analysis combined with a molecular dynamics simulation, Bresme and Quirke (1999) showed that line tension influences the wetting behavior of nanoparticles at liquid-vapor and liquid-liquid interfaces. These authors found negative line tension values for particles of a few nanometers in diameter, but positive values for those an order of magnitude A change in quantity or volume as measured by the decimal point. For example, from tens to hundreds is one order of magnitude. Tens to thousands is two orders of magnitude; tens to millions is three orders of magnitude, etc. larger. A negative line tension favors the initial wetting of a spherical particle after its approach to an interface. Shanahan (1990) studied the engulfment of solid-surface heterogeneities equivalent to particles in the nanometer range by unbalanced capillary forces (free energy perturbations). Thermal capillary waves cause fluid droplets to coalesce with a fluid substrate by film drainage at the interface, breakage of the film, and intrusion of the particle into the bulk phase (Aarts et al. 2004). Thus, thermal capillary fluctuations may enhance particle transport through cell membranes. Experimental results demonstrate consistently greater immersion of smaller particles than larger ones into a liquid substrate covered by surfactant film in vitro as well as in situ in airways. These results support the concept that line tension plays a significant role in particle displacement (Geiser et al. 2000; Schurch et al. 1999). It remains to be determined which chemical and physical properties of membranes and particles are responsible for the translocation of UFPs in vivo. Interestingly, we did not see any difference in particle uptake in vitro with respect to differing surface charges or surface chemistry when we used three different particle types: a metal, a metal oxide, and a synthetic polymeric material (data not shown). However, these particles were added to the cells in suspension and did not approach the cells from the air or require passage through a surfactant film first, as in the in vivo inhalation experiments. In these in vivo experiments, electrostatic interactions are likely important for particle deposition and subsequent retention. In summary, UFPs of various materials can cross any cellular membrane, but neither endocytosis, which is based on vesicle formation, nor any actin-based mechanisms are likely to account for UFP translocation into the cell. Our results from the inhalation experiments with Ti[O.sub.2] particles point to a transport mechanism that includes adhesive interactions or, in terms of thermodynamics, interfacial and line tension effects. In addition, particle diffusion and uptake promoted by thermal capillary waves might play a role in particle transport through membranes. After the deposition of nanometer-size particles, their further fate may be largely independent from particle surface chemistry and charge. Consequently, it is a possible fate of inhaled ambient UFPs that they are transferred from the lungs to most other organs. In a first analysis of ultrathin sections from hearts of the same rats, we found ultrafine Ti[O.sub.2] particles in the connective tissue, that is, within fibroblasts (data not shown). There may be no means on the cellular level to prevent, influence, or direct their uptake. Moreover, the toxic potential of UFPs is greatly enhanced by their free location and movement within cells, which promote interactions with intracellular proteins and organelles and even the nuclear DNA. Potential health implications of our findings are related not only to ambient UFPs but also to engineered "nanoscaled particles," which may be released into our environment during their production, transport, and aging, or during waste disposal (The Royal Society 2004). Routes of exposure to nanomaterials include oral, cutaneous cutaneous /cu·ta·ne·ous/ (ku-ta´ne-us) pertaining to the skin. cu·ta·ne·ous adj. Of, relating to, or affecting the skin. 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Marianne Geiser, (1) Barbara Rothen-Rutishauser, (1) Nadine Kapp, (1) Samuel Schurch, (1,2) Wolfgang Kreyling, (3) Holger Schulz, (3) Manuela Semmler, (3) Vinzenz Im Hof, (4) Joachim Heyder, (3) and Peter Gehr (1) (1) Institute for Anatomy, University of Bern The University of Bern is a university in the Swiss capital of Bern. It was founded in 1834. As one of the German-speaking universities in Switzerland its official name is Universität Bern, although it is frequently referred to in the French form, Université de Berne. , Bern, Switzerland; (2) Department of Physiology and Biophysics biophysics, application of various methods and principles of physical science to the study of biological problems. In physiological biophysics physical mechanisms have been used to explain such biological processes as the transmission of nerve impulses, the muscle , Faculty of Medicine, The University of Calgary, Calgary, Alberta, Canada; (3) GSF-National Research Center for Environment and Health, Institute for Inhalation Biology, Neuherberg/Munich, Germany; (4) Institute of Pathophysiology pathophysiology /patho·phys·i·ol·o·gy/ (-fiz?e-ol´ah-je) the physiology of disordered function. path·o·phys·i·ol·o·gy n. 1. , University of Bern, Bern, Switzerland Address correspondence to M. Geiser, Institute of Anatomy, University of Bern, Baltzerstrasse 2, CH-3000 Bern 9, Switzerland. Telephone: 41-31-631-8475. Fax: 41-31-631-3807. E-mail: geiser@ana.unibe.ch We thank S. Frank, B. Haenni, B. Kupferschmid, and B. Tschirren for excellent technical assistance and L.M. Cruz-Orive for his help with the lung sampling design. This study was supported by the Swiss National Science Foundation The Swiss National Science Foundation is a science research support organization mandated by the Swiss Federal Government. The SNSF was established in 1952 as a foundation under private law. Its secretariat is based in Berne. ; the Swiss Agency for the Environment, Forest, and Landscape; and the Silva Casa Foundation. The authors declare they have no competing financial interests. |
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