Mycotoxin adducts on human serum albumin: biomarkers of exposure to Stachybotrys chartarum.OBJECTIVE: Despite the growing body of evidence showing adverse health effects from inhalation exposure to the trichothecene-producing mold Stachybotrys chartarum, controversy remains. Currently, there are no reliable assays suitable for clinical diagnosis of exposure. We hypothesized that satratoxin G (SG)-albumin adducts may serve as biomarkers of exposure to this fungus. DESIGN: We studied the formation of adducts of SG with serum albumin in vitro using Western blots and mass spectrometry (MS) and searched for similar adducts formed in vivo using human and animal serum. RESULTS: Samples of purified human serum albumin that had been incubated with increasing concentrations of SG showed concentration-dependent albumin bands in Western blots developed with anti-SG antibodies. MS analysis found that as many as 10 toxin molecules can be bound in vitro to one albumin molecule. The sequencing of albumin-adduct tryptic tryp·tic adj. Relating to or resulting from trypsin. tryptic relating to or resulting from digestion by trypsin. peptides and the analysis of pronase/amino peptidase peptidase /pep·ti·dase/ (pep´ti-das) any of a subclass of proteolytic enzymes that catalyze the hydrolysis of peptide linkages; it comprises the exopeptidases and endopeptidases. pep·ti·dase n. digests demonstrated that lysyl, cysteinyl, and histidyl residues are involved in the formation of these adducts. Serum samples from three patients with documented exposure to S. chartarum similarly revealed lysine-, cysteine-, and histidine-SG adducts after exhaustive digestion, affinity column enrichment, and MS analysis. These adducts were also found in the sera from rats exposed to the spores of S. chartarum in contrast to control human subjects and control animals. CONCLUSIONS: These data document the occurrence of SG-albumin adducts in both in vitro experiments and in vivo human and animal exposures to S. chartarum. RELEVANCE TO CLINICAL PRACTICE: SG-amino acid adducts may serve as reliable dosimeter do·sim·e·ter n. An instrument that measures the amount of radiation absorbed in a given period. dosimeter an instrument used to detect and measure exposure to radiation. biomarkers for detection of exposure to S. chartarum. KEY WORDS: biomarkers, satratoxin G, Stachybotrys chartarum, trichothecenes. Environ Health Perspect 114:1221-1226 (2006). doi:10.1289/ehp.9064 available via http://dx.doi.org/ [Online 26 April 2006] ********** The filamentous mold Stachybotrys chartarum requires water-saturated cellulose to grow, and when found in an indoor environment, it is an indicator of significant water intrusion and damage. Although S. chartarum produces several classes of mycotoxins, of greatest concern are macrocyclic trichothecenes, the most potent members of a large family of trichothecenes (Miller et al. 2003). These mycotoxins bind to a single site on eukaryotic eukaryotic /eu·kary·ot·ic/ (u?kar-e-ot´ik) pertaining to a eukaryon or to a eukaryote. eukaryotic pertaining to eukaryosis. eukaryotic cells see cell. ribosomes Ribosomes Small particles, present in large numbers in every living cell, whose function is to convert stored genetic information into protein molecules. and directly inhibit initiation, elongation, or termination of protein synthesis depending on which trichothecene is bound (Feinberg and MacLaughlin 1989). There are two chemotypes of S. chartarum, one producing several macrocyclic trichothecenes and another that produces atranones and simple trichothecenes (e.g., trichodermin) but never any of the macrocyclic trichothecenes (Andersen et al. 2002). Although animal models of pulmonary injury demonstrate that macrocyclic trichothecenes are not the only source of lung damage, tracheal tracheal pertaining to or emanating from trachea. tracheal aspiration see transtracheal aspiration. tracheal band sign on contrast radiography of a dilated esophagus, the impression made ventrally by the trachea. instillation of spores containing these mycotoxins results in significantly more acute injury (Leino et al. 2003; Yike and Dearborn 2004; Yike et al. 2005). Concern about S. chartarum in indoor environments surfaced in the mid-1980s (Croft et al. 1986). Case reports of exposures in both residential and the nonindustrial workplace suggested that chronic indoor exposures could result in a variety of debilitating de·bil·i·tat·ing adj. Causing a loss of strength or energy. Debilitating Weakening, or reducing the strength of. Mentioned in: Stress Reduction respiratory and nonrespiratory symptoms, perhaps including an effect on immune function (Hodgson et al. 1998; Johanning et al. 1996). Recent reviews on toxic mold-related health effects raise both concern and controversy (Horner 2005; Hossain et al. 2004). In 1994 we recognized an outbreak of acute pulmonary hemorrhage in young infants in Cleveland (Montana et al. 1997). The initial case-control investigation led by the Centers for Disease Control and Prevention Centers for Disease Control and Prevention (CDC), agency of the U.S. Public Health Service since 1973, with headquarters in Atlanta; it was established in 1946 as the Communicable Disease Center. (CDC See Control Data, century date change and Back Orifice. CDC - Control Data Corporation ) found an association of this often fatal disorder with the presence of S. chartarum in the water-damaged homes of these infants (Etzel et al. 1998). Although subsequent review by the CDC of the initial field investigation of 10 infant cases and 30 controls has questioned the strength of the association (Etzel 2003), we have subsequently cared for an additional 30 cases with the continued observation that almost 90% of these infants come from homes with documented S. chartarum (Dearborn et al. 1999, 2002). Others have also seen pulmonary hemorrhage in infants with toxigenic toxigenic /tox·i·gen·ic/ (tok?si-jen´ik) 1. producing or elaborating toxins. 2. derived from or containing toxins. tox·i·gen·ic adj. Producing a poison; toxicogenic. mold exposure (Miller et al. 2003), and informal surveillance identified more than 100 other cases of acute infant pulmonary hemorrhage diagnosed across the United States between 1993 and 1997 (Dearborn et al. 1999). The non-pulmonary manifestations are similar to those described in animals exposed to S. chartarum and are consistent with the immune suppressive sup·pres·sive adj. Tending or serving to suppress. Adj. 1. suppressive - tending to suppress; "the government used suppressive measures to control the protest" , neurotoxic neurotoxic pertaining to or emanating from a neurotoxin. neurotoxic state a case of poisoning by a neurotoxin. neurotoxic adjective , and hemolytic he·mo·lyt·ic adj. Destructive to red blood cells; hematolytic. Hemolytic Referring to the destruction of the cell membranes of red blood cells, resulting in the release of hemoglobin from the damaged cell. effects of the trichothecenes and/or accompanying mycotoxins (Dearborn et al. 2002). Conclusive evidence regarding the etiology of the infant pulmonary hemorrhage disorder and other adverse health effects linked to exposure to this mold awaits the development of proper biomarkers. At present, there is no reliable way to determine human exposure to S. chartarum (Dillon et al. 1999; Miller et al. 2003). Finding this mold in a patient's home or work environment remains circumstantial evidence without a biological marker documenting the extent and timing of the exposure. Whether it is infants, older children, or adults, it is very apparent that the controversy surrounding the significance of inhalation exposure to "toxic mold" will continue until quantitative, dosimeter biomarkers are available and used in proper epidemiologic studies. In this report, we present evidence that satratoxin G (SG), a macrocyclic trichothecene produced by S. chartarum (Figure 1), forms covalent co·va·lent adj. Of or relating to a chemical bond characterized by one or more pairs of shared electrons. adducts with serum albumin. These adducts may serve as biomarkers of exposure to S. chartarum similar to the serum albumin adducts that have been used as exposure dosimeters for another mycotoxin mycotoxin Toxin produced by a fungus. Numerous and varied, mycotoxins can cause hallucinations, skin inflammation, liver damage, hemorrhages, miscarriage, convulsions, neurological disturbances, and/or death in livestock and humans. , aflatoxin B1, and other xenobiotics and chemicals (Groopman and Kensler 1999). Materials and Methods Experimental design. Figure 2 is a summary of the in vitro and in vivo experiments and analyses described in this article. Animal experiments. Animals. Sprague-Dawley rats were obtained from Charles River (Wilmington, MA). All animals were housed in microisolators in the Case Western Reserve University animal facility and fed the standard diet of Teklad 8664 (Harlan, Madison, WI) and water ad libitum. The animal research protocol has been approved by the Case Western Reserve University 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. . The animals were treated humanely and with regard for the alleviation of suffering. Intratracheal instillation of fungal spores. Seven-day-old rat pups weighing around 10 g were used for measurements of SG in blood. Male and female rats weighing 100 g were used to search for SG-albumin adducts. In both cases, the 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 with isoflurane (Baxter, Deerfield, IL). A transverse skin incision was made, and the trachea trachea (trā`kēə) or windpipe, principal tube that carries air to and from the lungs. It is about 4 1-2 in. (11.4 cm) long and about 3-4 in. (1.9 cm) in diameter in the adult. was exposed by blunt dissection. S. chartarum spores (isolate JS58-17; 4.0 x [10.sup.5] spores per gram body weight in SG measuring experiments and 0.5 x [10.sup.5] spores/gram body weight in albumin adduct adduct /ad·duct/ (ah-dukt´) to draw toward the median plane or (in the digits) toward the axial line of a limb. adduct /ad·duct/ (a´dukt) inclusion complex. detection experiments) suspended in 50 [micro]L of 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, ) containing 0.1% Tween-20 were injected directly into the trachea using a 24 G angiocatheter attached to a sterile Hamilton syringe. The incision was closed and treated with New Skin liquid bandage (Medtech Laboratories Inc., Jackson, WY) to facilitate healing. Collection of blood. The animals were exsanguinated through the right ventricle under isoflurane anesthesia at indicated times after spore instillation, and the blood samples were combined using three animals per time point. For SG measurements, the blood was immediately extracted with ethanol (see below), whereas for albumin adduct detection, the blood was centrifuged at 1,000 x g for 10 min and the serum aspirated and stored at -20[degrees]C. Human blood samples. Blood samples were obtained from three adult patients with documented exposure to S. chartarum who were evaluated at the Environmental Health Clinic, Swetland Center for Environmental Health, Case Western Reserve University (Cleveland, OH). The use of human samples was reviewed and approved by the Institutional Review Board of the University Hospitals of Cleveland University Hospitals is a major not-for-profit medical center in Cleveland, Ohio, United States. With 150 locations throughout northeast Ohio, it encompasses a network of hospitals, outpatient centers and primary care physicians. , and all recruited patients gave informed consent. The sample from patient 1 was taken approximately 2 months after the completion of mold remediation in her home. Previous air sampling in her living room had measured 4,700 S. chartarum spores/[m.sup.3] (Air-O-Cell; US Micro-Solutions Inc, Greensburg, PA). Blood samples from patients 2 and 3 were obtained while they were still living in their home where S. chartarum was found in their bedroom carpeting (1,030 S. chartarum spore equivalents/g; quantitative polymerase chain reaction Quantitative polymerase chain reaction (qPCR) is a modification of the polymerase chain reaction used to rapidly measure the quantity of DNA, complementary DNA or ribonucleic acid present in a sample. , P & K Microbiology Services, Cherry Hill, NJ). Control blood samples were received from the investigators. The blood was centrifuged and the serum stored at -20[degrees]C. Anti-SG antibodies and SG ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. . Polyclonal antibodies against SG were generously donated by J. Pestka, Michigan State University Michigan State University, at East Lansing; land-grant and state supported; coeducational; chartered 1855. It opened in 1857 as Michigan Agricultural College, the first state agricultural college. (East Lansing, MI). The IgG fraction, obtained by ammonium sulfate precipitation Ammonium sulfate precipitation is a method of protein purification by altering solubility of protein. It is a specific case of a more general technique known as salting out. from the sera of rabbits immunized with the conjugates of bovine serum albumin and SG (Chung et al. 2003), was purified by passing through an affinity column of bovine serum albumin (Sigma-Aldrich, St. Louis, MO) conjugated conjugated adj. Conjugate. estrogens, conjugated Warning - Hazardous drug! C.E.S. to Amino Link Sepharose (Pierce, Rockford, IL) to remove antibodies specific for bovine albumin epitopes. SG was measured by ELISA (detection limit = 0.1 ng/mL) in 1:1 whole blood ethanol extracts according to the method of Chung et al. (2003) using anti-SG antibody and horseradish horseradish Hardy perennial plant (Armoracia lapathifolia) of the mustard family, native to Mediterranean lands and grown throughout the temperate zones. Its hotly pungent, fleshy root is used as a condiment and is traditionally considered medicinal. peroxidase-SG conjugates provided by J. Pestka. Formation of albumin-SG adducts in vitro. Human serum albumin (HSA HSA Health Savings Account (US) HSA Human Serum Albumin HSA Human Services Agency (Nevada) HSA Health Services Agency HSA Health and Safety Authority (Ireland) ) isolated from human blood (Sigma-Aldrich) and/or recombinant HSA (rHSA; GTC GTC See: Good 'til cancelled order GTC See good-till-canceled order (GTC). Biotherapeutics, Spencer, MA) was dissolved in PBS at 10 [micro]M concentration and incubated for 20 hr at 37[degrees]C with 0-, 1-, 2-, 5-, 10-, and 20-molar excess of SG (gift from B. Jarvis, University of Maryland University of Maryland can refer to:
sodium dodecyl sulfate-polyacrylamide gel electrophoresis. followed by Western blots or dialyzed di·a·lyze tr. & intr.v. di·a·lyzed, di·a·lyz·ing, di·a·lyz·es To subject to or undergo dialysis. [Back-formation from dialysis. and analyzed by mass spectrometry (MS) as described below. A molar ratio of 1:10 of albumin to SG was used for MS studies. N-[alpha]-Acetyl-L-lysine (Sigma-Aldrich) was dissolved in PBS at 10 [micro]M concentration and incubated for 20 hr at 37[degrees]C with an equimolar e·qui·mo·lar adj. Chemistry Having an equal number of moles. concentration of SG. Electrophoresis and Western blot analysis West·ern blot analysis n. An electrophoretic procedure for separating proteins. . SDS-PAGE was performed using 12% precast pre·cast adj. Relating to or being a structural member, especially of concrete, that has been cast into form before being transported to its site of installation. Criterion gels (Bio-Rad, Hercules, CA). The proteins were transferred to nitrocellulose nitrocellulose, nitric acid ester of cellulose (a glucose polymer). It is usually formed by the action of a mixture of nitric and sulfuric acids on purified cotton or wood pulp. , and Western blots were developed using 1:1,000-diluted (affinity purified as above) anti-SG antibody. Alkaline phosphatase anti-rabbit IgG (Sigma-Aldrich) was used as a secondary antibody, and the protein bands were visualized with an alkaline phosphatase substrate kit (Bio-Rad). Preparation of samples for MS analysis Tryptic digestion of rHSA and human serum. rHSA was incubated with (1:10 molar ratio of rHSA to SG) and without SG as described above and dialyzed against 20 mM ammonium bicarbonate, pH 7.8. Dialyzed protein was incubated overnight at 37[degrees]C with sequencing-grade trypsin trypsin, enzyme that acts to degrade protein; it is often referred to as a proteolytic enzyme, or proteinase. Trypsin is one of the three principal digestive proteinases, the other two being pepsin and chymotrypsin. (Promega, Madison, WI) at 1:100 wt/wt ratio. Samples of human serum (1-3 mL) were similarly digested with a TCPK trypsin preparation (Sigma-Aldrich). Exhaustive digestion of rHSA and serum. rHSA and rHSA-SG adducts, dialyzed overnight against 20 mM ammonium bicarbonate pH 7.8, were incubated overnight at 37[degrees]C with pronase (Calbiochem, EMD EMD Electromechanical dissociation, see there Biosciences, San Diego, CA) at 1:100 wt/wt ratio and leucine leucine (l  `sēn), organic compund, one of the 20 amino acids commonly found in animal proteins. aminopeptidase a·mi·no·pep·ti·dasen. Any of various enzymes that catalyze the hydrolysis of the terminal peptide bond at the amino end of a polypeptide. aminopeptidase (Sigma-Aldrich) at 1:1,000 wt/wt ratio. Human and rat serum (1-3 mL) were similarly digested except using the leucine aminopeptidase at 1:500 wt/wt. If the digestion to single amino acids was not complete, carboxypeptidase carboxypeptidase /car·boxy·pep·ti·dase/ (-pep´ti-das) any exopeptidase that catalyzes the hydrolytic cleavage of the terminal or penultimate bond at the end of a peptide or polypeptide where the free carboxyl group occurs. Y (Sigma-Aldrich) was added to reconstituted samples for 4 hr and the analysis was repeated. Affinity chromatography. Both trypsin and pronase digested samples were heat inactivated inactivated rendered inactive; the activity is destroyed. inactivated viruses treated so that they are no longer able to produce evidence of growth or damaging effect on tissue. at 60[degrees]C for 30 min and centrifuged at 17,000 x g for 20 min before affinity chromatography. The affinity column for isolating peptide and amino acid adducts was prepared by conjugating anti-SG antibody (see above) to AminoLink Sepharose (Pierce, Rockford, IL). Heat-inactivated tryptic and/or pronase digests from human and rat serum were loaded onto the column and incubated for 1 hr at room temperature. The column was extensively washed with PBS followed by 20 mM ammonium bicarbonate, pH 7.8. Bound adducts were eluted with 0.02% formic acid and evaporated. The samples were reconstituted in 0.1% formic acid and analyzed by MS. MS instrumentation and analyses. Intact protein. Intact rHSA was analyzed using an Applied Biosystems (Framingham, MA) Q-STAR XL quadrupole A quadrupole is one of a sequence of configurations of electric charge or gravitational mass that can exist in ideal form, but it is usually just part of a multipole expansion of a more complex structure reflecting various orders of complexity. time-of-flight (TOF (Top Of Form) The beginning of a physical paper form. To position paper in many printers, the printer is turned offline, the forms are aligned properly and the TOF button is pressed. ) mass spectrometer equipped with a nanospray source or a Bruker (Billerica, MA) Biflex III TOF mass spectrometer with a matrix-assisted laser desorption Desorption A process in which atomic and molecular species residing on the surface of a solid leave the surface and enter the surrounding gas or vacuum. ionization (MALDI MALDI Matrix-Assisted Laser Desorption/Ionization ) source. For intact protein analysis by MALDI-TOF-MS, sinapinic acid was used as the matrix. One microliter microliter /mi·cro·li·ter/ (µL) (mi´kro-le?ter) one millionth (10-6) of a liter. mi·cro·li·ter n. A unit of volume equal to one-millionth (10-6) of a liter. of the saturated matrix mixture (in a 1:1 acetonitrile acetonitrile /ac·e·to·ni·trile/ (as?e-to-ni´tril) a colorless liquid with an etherlike odor used as an extractant, solvent, and intermediate; ingestion or inhalation yields cyanide as a metabolic product. : water solution) was spotted on target with 1 [micro]L of the protein solution. Tryptic peptide identification. After rHSA digestion with trypsin, the resulting peptides were analyzed using MALDI-TOF-MS to determine their molecular weights. For MALDI-TOF-MS analysis of the peptides, the matrix [alpha]-cyano-4-hydroxy cinnamic acid was used. One microliter of the saturated matrix (in a 1:1 acetonitrile:water solutions) was spotted on target with 1 [micro]L of the analyte. Using the m/z values from the mass spectra, peptide mass fingerprinting Peptide mass fingerprinting (PMF) (also known as protein fingerprinting) is an analytical technique for protein identification that was developed 1993 by several groups independently. (PMF PMF, n.pr See proprioceptive neuromuscular facilitation. ) was performed to determine the identity of the peptides by matching the experimental molecular weights with the theoretical values calculated from the protein sequence. To further confirm the identity of the peptides and locate the modified amino acids, tandem MS (MS-MS) was performed using the ThermoElectron ther·mo·e·lec·tron n. An electron emitted by a material at high temperatures. LCQ-Deca XP (Thermo-Electron Corp., Waltham, MA) plus ion trap mass spectrometer with nanospray source. Tryptic digests were diluted in 1% acetic acid, and 2 [micro]L of each sample were pressure injected onto a self-packed 10 cm x 75 [micro]m innerdiameter Phenomenex Jupiter (Phenomenex Inc., Torrance, CA) [C.sub.18] reversed-phase capillary column. The peptides were eluted from the column by an acetonitrile and aqueous 0.05 M acetic acid gradient with a flow rate of approximately 0.25 [micro]L/min at the nanospray tip. The digest was analyzed by acquiring full scan mass spectra followed by MS-MS. The three most abundant ions detected in the full scan mass spectrum were then selected and fragmented to yield the MS-MS spectrum of the peptide. The MS-MS data were analyzed using the ThermoElectron BioWorks 3.1 program (ThermoElectron). All matching spectra were verified manually. The pronase digests were analyzed on the MALDI-TOF MALDI-TOF Matrix Assisted Laser Desorption Ionization - Time of Flight mass spectrometer using the same matrix and sample preparation detailed above for the tryptic digest analysis. The limit of detection for this analysis of human samples was approximately 10 nmol/mL of serum. Results Detection of SG in blood. When 7-day-old infant rat pups were exposed intratracheally to high doses (4.0 x [10.sup.5] spores/gm body weight) of highly toxic S. chartarum (isolate JS58-17), SG was detected in ethanol extracts of the whole blood by SG ELISA only immediately after instillation (Figure 3). The level of free toxin decreased below the detection limit within the next 15 min. No immunoreactive immunoreactive exhibiting immunoreactivity. free toxin could be detected in the sera of exposed animals between 1 and 72 hr postexposure. SG adducts in vitro. Detection of anti-SG-reactive albumin. Samples of purified HSA (Sigma-Aldrich) were incubated with increasing concentrations of SG (PBS, 37[degrees]C, 20 hr) and subjected to SDS-PAGE after reduction and boiling of the samples. Western blots using anti-SG antibody clearly demonstrate the HSA band at approximately 67 kDa (Figure 4) with the intensity of staining increasing with increasing concentrations of SG. This concentration dependence of the SG staining that persists through boiling and SDS 1. (company) SDS - Scientific Data Systems. 2. (tool) SDS - Schema Definition Set. electrophoresis supports the formation of covalent SG-albumin adducts. These results were confirmed using rHSA. MS analysis of intact protein. When untreated and SG-incubated rHSA (20 hr, 37[degrees]C, PBS, 1:10 protein to toxin ratio) were analyzed using an electrospray ionization (ESI (Edge Side Includes) A markup language for Web pages that enables elements of a Web page to be dynamically assembled in servers distributed throughout the Internet. ) ESI-quadrupole TOF mass spectrometer, a mass shift was seen in the treated rHSA sample. This molecular weight increase was indicative of as many as 10 satratoxin molecules bound to the protein. These results were further confirmed using a MALDI-TOF mass spectrometer (data not shown). MS analysis of SG-N-acetyl-L-lysine adduct. Because the [epsilon]-amines of lysyl residues are a likely site of SG nucleophilic attack, we incubated the toxin with N-[alpha]-acetyl-L-lysine (1:1 molar ratio, 37[degrees]C, 20 hr) and analyzed the resulting SG-lysyl adduct. Figure 5A and B, shows the spectra from both MALDI-TOF and ESI MS-MS of the resulting SG-lysyl adduct. The m/z 716 is consistent with the addition of 528 Da, an apparent loss of oxygen when the SG bound to the amino acid. When the ions at m/z 716 were isolated and fragmented, the MS/MS MS/MS Tandem Mass Spectroscopy MS/MS Multistage Mass Spectrometry spectrum contained a peak at m/z 172 representing the N-acetyl lysine lysine (lī`sēn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. as well as a peak representing a fragment of the toxin at m/z 239, a convenient marker for this adduct in MS-MS experiments. This peak at 239 Da is detected both in the mass spectrum of the toxin molecule alone and as a fragment ion in the MS-MS spectrum of the toxin molecule. Detection of adducted tryptic peptides from rHSA. To locate the sites of SG adduction adduction /ad·duc·tion/ (ah-duk´shun) the act of adducting; the state of being adducted. adduction ( to rHSA, both untreated and treated rHSA were digested with trypsin and analyzed with MALDI-TOF MS using PMF to identify the peptides. When analyzing the tryptic peptides of treated rHSA, several ions were detected that were consistent with the predicted mass of peptides bound to one SG molecule (Table 1). To identify the exact position of toxin molecules on these peptides, the tryptic digests of treated and control rHSA were analyzed further using ESI MS-MS (Table 1, Figure 6). Around 60% coverage was obtained for both samples. The ions representing tryptic peptides were in the triply charged state. When the ions at m/z 528 were isolated and fragmented, the resulting MS-MS spectrum identified the peptide as K(SG528)YLYEIAR with a calculated mass of 1,582 [(528 x 3) - 2]. Another labeled peptide was identified when the ions at m/z 475 were isolated and fragmented. The fragmentation pattern in this MS-MS spectrum is consistent with the peptide LC(SG544)TVATLR with a calculated mass of 1,423 Da [(475 x 3) - 2]. Last, when the ions at m/z 469 were fragmented, the same peptide was identified, but with a +528 SG adduct [(469 x 3) - 2] = 1,405 Da. As indicated in Table 1, the sequences of adducted tryptic peptides all contained lysyl, cysteinyl, or histidyl residues (see below), residues that are likely to be susceptible to modification by the toxin epoxide epoxide /epox·ide/ (e-pok´sid) an organic compound containing a reactive group resulting from the union of an oxygen atom with two other atoms, usually carbon, that are themselves joined together. groups. Detection of adducted amino acids in pronase digests of rHSA. To further characterize the rHSA-SG reactivity, exhaustive proteolysis proteolysis Process in which a protein is broken down partially, into peptides, or completely, into amino acids, by proteolytic enzymes, present in bacteria and in plants but most abundant in animals. of reacted rHSA was performed with pronase and leucine aminopeptidase. The modified amino acids were purified using anti-SG antibody affinity chromatography and analyzed by MALDI-TOF-MS. In the MALDI-TOF mass spectra, several ions were detected corresponding to the amino acids lysine (Lys), histidine histidine (hĭs`tĭdēn), organic compound, one of the 22 α-amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. (His), and cysteine cysteine (sĭs`tēn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer participates in the biosynthesis of mammalian protein. (Cys), each containing one SG molecule (Figure 7A). Two different cysteinyl adducts of +528 and +544 Da were detected. The amino acid assignments in Figure 7A were confirmed by ESI MS-MS (data not shown). SG-albumin adducts in vivo. Amino acid SG adducts in pronase digests of human and rat sera. Subsequently, 2 mL serum samples from three patients with documented exposure to S. chartarum and three control subjects were digested with pronase and leucine aminopeptidase, and the adducts were affinity purified and analyzed by MALDI-TOF MS. In Figure 7B, the three top spectra in each panel were acquired from the samples from exposed patients, whereas the bottom spectra are from one of the control subjects. Patients 2 and 3 had a more recent exposure compared to patient 1. Although cysteinyl adducts were detected in all three of the exposed patient samples, lysyl and histidyl adducts were not detected in patient 1, whose blood sample was collected 2 months after the termination of exposure. No amino acid adducts were detected in the sera from the three control subjects. Similarly, cysteine-, lysine-, and histidine-SG adducts were detected after exhaustive proteolysis of the sera of rats exposed intratracheally to S. chartarum collected 6 hr after the instillation of fungal spores (Figure 8). No adducts could be found in parallel samples from control animals. Adducted tryptic peptides from serum of a patient exposed to S. chartarum. To demonstrate the albumin origin of amino acid adducts detected in samples from human subjects, serum from patient 3 (most recent exposure, all three amino acyl ac·yl n. A organic radical having the general formula RCO, derived from the removal of a hydroxyl group from an organic acid. acyl 1. an organic radical derived from a fatty acid by removal of the hydroxyl group. 2. adducts detected) was digested with trypsin and the adducted peptides isolated with anti-SG immunoaffinity chromatography. Analysis by MALDI-TOF-MS followed with PMF detected eight peptides with the additional mass of 528 Da and four with 544 Da (Table 2). All of the detected tryptic peptides contained at least one of the three amino acyl residues, lysyl, cysteinyl, and histidyl, that were identified as probable modification sites in rHSA. Discussion In this study we have demonstrated that SG, a macrocylic trichothecene produced by S. chartarum, forms covalent adducts with HSA and that these adducts can be detected in clinical samples from patients exposed to this fungus. Serum albumin adducts have been used as exposure dosimeters for other toxic agents including another mycotoxin, aflatoxin B1 (Groopman and Kensler 1999; Guengerich et al. 2002; Sabbioni et al. 1990). This potent carcinogen causing hepatocellular carcinoma is oxidized oxidized having been modified by the process of oxidation. oxidized cellulose see absorbable cellulose. in the liver by cytochrome P450 to the epoxide that then reacts with the [epsilon]-amine of lysyl residues either directly or through the spontaneously formed dialdehyde. The five primary macrocyclic trichothecenes produced by S. chartarum are SG (Figure 1), satratoxin H, isosatratoxin F, roridin E, and verrucarin J. All contain an epoxide group that is critical to their toxicity, and the first and third of this series contain a second epoxide (Andersen et al. 2002; Jarvis et al. 1998). These highly reactive groups are likely to be involved in rapid adduct formation with proteins, and with inhalation exposure, this reaction would likely occur with blood proteins in the alveolar alveolar /al·ve·o·lar/ (al-ve´o-lar) [L. alveolaris ] pertaining to an alveolus. al·ve·o·lar adj. Relating to an alveolus. capillaries. The formation of mycotoxins adducts is consistent with our observation that free SG could be detected in the blood of rat pups exposed to the spores of S. chartarum only immediately after exposure (Figure 3), and with previous observations of rapid removal and/or metabolism of trichothecenes (Swanson and Corley 1989). Reaction with serum albumin and other blood proteins is likely responsible for the rapid disappearance of free toxin from the blood. The reaction of SG with tissue and cellular proteins is also likely. Our first experimental data suggesting the formation of SG-protein adducts was the detection of immunoreactive satratoxin in murine tissue sections and cells obtained by bronchoalveolar lavage. The presence of satratoxin epitopes in lung sections that had been extensively rinsed in organic solvents during fixation and staining (Gregory et al. 2004) indicated that the toxin might be covalently bound to tissue/cell components. Western blots showing the staining of albumin with anti-SG antibody (Figure 4) were obtained with reduced and boiled samples, further suggesting covalent links between the mycotoxin and protein. ESI TOF and MALDI-TOF-MS analysis of the intact adducted protein showed that up to 10 amino acid residues in the albumin molecule are modified after the incubation of the protein with a 20-fold excess of toxin in vitro. The extent of albumin modification in vivo would be dependent upon the level and timing of exposure and is likely to reflect the cumulative nature of chronic exposure. MALDI-TOF-MS analysis of exhaustive pronase/aminopeptidase digests of rHSA demonstrated that in addition to lysyl residues, two other amino acyl residues, cysteinyl and histidyl, are involved in adduct formation. All of the rHSA-derived tryptic peptides with SG adducts had one of those amino acyl residues within their sequences, and Cys75 and Lys137 were positively identified as modification sites using ESI MS-MS analysis. Using an affinity column with anti-SG antibodies to isolate adducts from proteolytic pro·te·o·lyt·ic adj. Relating to, characterized by, or promoting proteolysis. proteolytic (pro″teolit´ik), adj digests provides a concentrating step that greatly increases the sensitivity of detection. Our ability to detect Lys-, Cys-, and His-SG adducts in pronase/aminopeptidase digests of serum from patients exposed to S. chartarum in their homes, in contrast to samples from people without mold exposure, demonstrates the feasibility of a practical biomarker assay. Detection of modified tryptic peptides with albumin sequences in the sample of patient's serum indicates that those amino acyl adducts came from serum albumin, although modification of other serum proteins is likely. In addition, the presence of Lys-, Cys-, and His-SG adducts in the sera from rats exposed intratracheally to the spores of a highly toxic isolate of S. chartarum further confirms the biomarker potential of the adducts. An SG ELISA [the same assay developed by Chung et al. (2003) used in this study to measure SG in blood, as described in "Materials and Methods"] was used by Brasel et al. (2004) to detect the toxin in organic solvent extracts of the sera of patients exposed to molds through indoor air inhalation. Their removal of proteins before analysis precludes the detection of albumin-toxin adducts, although some amino acid and small peptide toxin adducts may be present in those extracts. Most of their positive clinical samples contained immunoreactive toxin very close to the limit of detection. MS analysis detected possible toxin breakdown products with spectral properties similar to those of macrocyclic trichothecenes, but the exact nature and origin of the detected substance are not known. For this approach to be quantitatively useful in assessing S. chartarum exposure, the nature and kinetics of SG metabolism in humans must be better understood. In addition, our animal experiments showing rapid loss of detectable free toxin from the blood after inhalation-type exposure suggest this analytical approach to be of limited value. Other methods to document S. chartarum exposure include reverse-transcriptase polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is (RT-PCR RT-PCR reverse transcriptase-polymerase chain reaction. See PCR1. ) using species-specific genomic probes and an ELISA for a hemolysin hemolysin /he·mol·y·sin/ (he-mol´i-sin) a substance that liberates hemoglobin from erythrocytes by interrupting their structural integrity. he·mol·y·sin n. produced by this fungus. Although quantitative PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) is quite sensitive (Haugland et al. 1999), the collection of proper secretion samples often requires invasive procedures (e.g., bronchoscopy Bronchoscopy Definition Bronchoscopy is a procedure in which a cylindrical fiberoptic scope is inserted into the airways. This scope contains a viewing device that allows the visual examination of the lower airways. ) in order to collect secretions likely to contain the fungus, which is also a time-limited sampling opportunity. In addition, detection using RT-PCR does not discriminate between the isolates that produce macrocyclic trichothecenes and those that do not. Similarly, the use of the hemolysin as a biomarker does not distinguish between macrocyclic trichothecene producers and non-producers because all of the tested isolates of S. chartarum seem to produce stachylysin (Vesper et al. 1999, 2001). The polyclonal antibodies currently used in the Stachylysin-ELISA assay (Van Emon et al. 2003) recognize fungal antigens from other species, such as Penicillium chrysogenum (Yike I, unpublished data). A more specific, monoclonal antibody may be needed in order to develop a reliable assay. A monoclonal antibody developed recently against a spore-specific antigen from S. chartarum recognizes a secreted protein found both in highly toxic isolates and in those with low toxicity. However, because of its relatively low abundance, this protein may be difficult to detect in human samples (Schmechel et al. 2006). Although the exact structures and mechanisms of the SG adduct formation require further studies, our ability to detect these adducts in blood samples of individuals and animals exposed to S. chartarum in contrast to control subjects indicates a high potential for this approach to provide a practical, quantitative dosimeter. Serum albumin is one of the most abundant proteins (~60 mg/mL) with a half-life of approximately 20 days. This makes it a good candidate for a dosimeter of both acute (days) and fairly recent (weeks to several months) mold exposure. Our results suggest that SG-albumin adducts may serve as quantitative biomarkers of inhalation exposure to S. chartarum and other satratoxin-producing fungi because they can be readily detected in small samples of blood. REFERENCES Andersen B, Nielsen KF, Jarvis BB. 2002. Characterization of Stachybotrys from water-damaged buildings based on morphology, growth, and metabolite metabolite, organic compound that is a starting material in, an intermediate in, or an end product of metabolism. Starting materials are substances, usually small and of simple structure, absorbed by the organism as food. production. Mycologia 94:392-403. Biemann, K. 1990. Nomenclature for peptide fragment ions (positive ions). Methods Enzymol 193:886-887. Brasel TL, Campbell AW, Demers RE, Ferguson BS, Fink J, Vojdani A, et al. 2004. Detection of trichothecene mycotoxins in sera from individuals exposed to Stachybotrys chartarum in indoor environments. Arch Environ Health 59:317-323. Chung YJ, Jarvis BB, Tak H, Pestka JJ. 2003. Immunochemical assay for satratoxin G and other macrocylcic trichothecenes associated with indoor air contaminination by Stachybotrys chartarum. Toxicol Mech Methods 13:1-7. Croft WA, Jarvis BB, Yatawara CS. 1986. Airborne outbreak of trichothecene toxicosis toxicosis /tox·i·co·sis/ (tok?si-ko´sis) any diseased condition due to poisoning. tox·i·co·sis n. pl. tox·i·co·ses 1. Systemic poisoning. 2. . Atmos Environ 20:549-552. Dearborn DG, Dahms BB, Allan TM, Sorenson WG, Montana E, Etzel RA. 2002. Clinical profile of 30 infants with acute pulmonary hemorrhage in Cleveland. Pediatrics 110:627-637. Dearborn DG, Yike I, Miller MJ, Etzel RA. 1999. An overview of the investigation into pulmonary hemorrhage in infants in Cleveland, Ohio. Environ Health Perspect 107(suppl 3):495-499. Dillon HK, Miller JD, Sorenson WG, Douwes J, Jacobs RR. 1999. Review of methods applicable to the assessment of mold exposure to children. Environ Health Perspect 107(suppl 3):473-480. Etzel RA. 2003. Stachybotrys. Curr Opin Pediatr 15:103-106. Etzel RA, Montana E, Sorenson WG, Kullman J, Allan TM, Dearborn DG. 1998. Acute pulmonary hemorrhage in infants associated with exposure to Stachybotrys atra and other fungi. Arch Pediatr Adolesc Med 152:757-762. Feinberg B, MacLaughlin CS. 1989. Biochemical mechanism of action of trichothecene mycotoxins. In: Trichothecene Mycotoxins: Pathophysiologic Effects (Beasley VR, ed). Vol 1. Boca Raton, FL:CRC (Cyclical Redundancy Checking) An error checking technique used to ensure the accuracy of transmitting digital data. The transmitted messages are divided into predetermined lengths which, used as dividends, are divided by a fixed divisor. Press, 27-36. Gregory L, Pestka J, Dearborn D, Rand TG. 2004. 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. of satratoxin-G in Stachybotrys chartarum spores and spore impacted mouse lung using immunocytochemistry im·mu·no·cy·to·chem·is·try n. The study of cell constituents by immunologic methods, such as the use of fluorescent antibodies. immunocytochemistry . Toxicol Pathol 32:26-34. Groopman JD, Kensler TW. 1999. The light at the end of the tunnel for chemical-specific biomarkers: daylight or headlight? Carcinogenesis 20:1-11. Guengerich FP, Arneson KO, Williams KM, Deng Z, Harris TM. 2002. Reaction of aflatoxin B1 oxidation products with lysine. Chem Res Toxicol 15:780-792. Haugland RA, Vesper SJ, Wymer LJ. 1999. Quantitative measurement of Stachybotrys chartarum conidia co·nid·i·a n. Plural of conidium. using real time detection of PCR products with the TaqMan[TM] fluorogenic probe system. Mol Cell Probes 13:329-340. Hodgson MJ, Morey P, Wing-Yan L, Morrow L, Miller D, Jarvis BB, et al. 1998. Building associated pulmonary disease from exposure to Stachybotrys chartarum and Aspergillus Aspergillus Any fungus of the genus Aspergillus of the Fungi Imperfecti (form-class Deuteromycetes). Species for which the sexual phase is known are placed in the order Eurotiales. A. niger causes black mold on some foods; A. niger, A. flavus, and A. versicolor versicolor /ver·si·co·lor/ (ver?si-kol´er) variegated; having a variety of colors, or changing in color. . J Occup Environ Med 40:241-249. Horner WE. 2005. The damp building effect: understanding needed, not more debate. Ann Allergy Asthma Immunol 94:213-215. Hossain MA, Ahmed MS, Ghannoum MA. 2004. Attributes of Stachybotrys chartarum and its association with human disease. J Allergy Clin Immunol 113:200-208. Jarvis BB, Sorenson WG, Hintikka E-L, Nikulin M, Zhou Y, Yang J, et al. 1998. Study of toxin production by isolates of Stachybotrys chartarum and Memnoniella echinata isolated during a study of pulmonary hemosiderosis in infants. Appl Environ Microbiol 64:3620-3625. Johanning E, Biagini R, Hull D, Morey P, Jarvis B, Landsbergis P. 1996. Health and immunology study following exposure to toxigenic fungi (Stachybotrys chartarum) in a water-damaged office environment. Int Arch Occup Environ Health 68:207-218. Leino M, Makela M, Reijula T, Haathela T, Mussalo-Rauhamaa H, Hintikka E-L, et al. 2003. Intranasal exposure to a damp building mold, Stachybotrys chartarum, induces lung inflammation in mice by satratoxin independent mechanisms. Clin Exp Allergy 33:1603-1610. Miller JD, Rand TG, Jarvis BB. 2003. Stachybotrys chartarum: a really malicious mold. Med Mycol 41:271-291. Montana E, Etzel RA, Allan TM, Horgan TE, Dearborn DG. 1997. Environmental risk factors associated with pediatric pediatric /pe·di·at·ric/ (pe?de-at´rik) pertaining to the health of children. pe·di·at·ric adj. Of or relating to pediatrics. idiopathic pulmonary hemosiderosis idiopathic pulmonary hemosiderosis n. Repeated attacks of difficulty in breathing and hemoptysis leading to the deposition of abnormal amounts of hemosiderin in the lungs. Also called Ceelen-Gellerstadt syndrome. in a Cleveland community. Pediatrics 99(1):e5. Available: http://www.pediatrics.org/cgi/content/full/99/1/e5 [accessed 04/11/06]. Sabbioni G, Ambs S, Wogan GN, Groopman JD. 1990. The aflatoxin-lysine adduct quantified by high-performance liquid chromatography from human serum albumin samples. Carcinogenesis 11:2063-2066. Schmechel D, Simpson JP, Beezhold D, Lewis DM. 2006. The development of species-specific immunodiagnostics for Stachybotrys chartarum: the role of cross-reactivity. J Immunol Methods 309:150-159. Swanson SP, Corley RA. 1989. The distribution, metabolism, and excretion of trichothecene mycotoxins. In: Trichothecene Mycotoxins: Pathophysiologic Effects (Beasley VR, ed). Vol 1. Boca Raton, FL:CRC Press, 37-62. Van Emon JM, Reed AW, Yike I, Vesper SJ. 2003. Measurement of Stachylysin[TM] in serum to quantify human exposures to the indoor mold Stachybotrys chartarum. J Occup Environ Med 45:582-591. Vesper SJ, Dearborn DG, Yike I, Sorenson WG, Haugland RA. 1999. Hemolysis hemolysis (hĭmŏl`ĭsĭs), destruction of red blood cells in the bloodstream. Although new red blood cells, or erythrocytes, are continuously created and old ones destroyed, an excessive rate of destruction sometimes occurs. , toxicity and RAPD RAPD Randomly Amplified Polymorphic DNA RAPD relative afferent pupillary defect (ophthalmology; aka Marcus-Gunn Pupil) analysis of Stachybotrys chartarum strains from the Cleveland pulmonary hemorrhage outbreak and non-Cleveland strains. Appl Environ Microbiol 65:3175-3181. Vesper SJ, Magnuson S, Dearborn D, Yike I, Haugland RA. 2001. Initial characterization of the hemolysin from Stachybotrys chartarum. Infect Immun 69:912-916. Yike I, Dearborn DG. 2004. Pulmonary effects of Stachybotrys chartarum in animal studies. Adv Appl Microbiol 55:241-273. Yike I, Rand T, Dearborn DG. 2005. Acute inflammatory responses to Stachybotrys chartarum in the lungs of infant rats: time course and possible mechanisms. Toxicol Sci 84:408-417. Iwona Yike, (1,3) Anne M. Distler, (2) Assem G. Ziady, (1) and Dorr G. Dearborn (1,3) Departments of (1) Pediatrics and (2) Pharmacology, and (3) Mary Ann Swetland Center for Environmental Health, Case Western Reserve University, Cleveland, Ohio, USA Address correspondence to D.G. Dearborn, Swetland Center for Environmental Health, Case Western Reserve University, School of Medicine, 10900 Euclid Ave., Cleveland, OH 44106-4948 USA. Telephone: (216) 368-8521. Fax: (216) 368-4518. E-mail: dxd9@case.edu We thank C. Hoppel and M. Chance for helpful discussions and J. Gower for excellent technical assistance. This work was supported by the Swetland Endowment, the Case Provost Opportunity Fund, and National Institutes of Health Metabolic training grant T23 DK007319 (A.M.D.). The authors declare they have no competing financial interests. Received 2 February 2006; accepted 26 April 2006.
Table 1. Adducted tryptic peptides from rHSA.
Amino
m/z acids Sequence (a) Adduct
5739.9 277-323 EC#C#EK#PLLEK#SH#C#IAEVENDEMPADLPSLAADFVESK#DV 528
C#K#NYAEAK
4566.2 214-276 VH#TEC#C#H#GDLLEC#ADDRADLAK#YIC#ENQDSISSK#LK 544
4565.2 485-519 RPC#FSALEVDETYVPK#EFNAETFTFH#ADIC#TLSEK 528
3487.5 82-106 ETYGEMADC#C#AK#QEPERNEC#FLQH#K 528
2551.5 223-240 FPK#AEFAEVSK#LVTDLTK 528
2551.5 467-484 TPVSDRVTK#C#C#TESLVNR 544
1914.5 263-274 YIC#ENQDSISSK 528
1582.6 137-144 K#*YLYEIAR 528
2583.3 145-160 RH#PYFYAPELLFFAK#R 528
2743.4 175-195 AAC#LLPK#LDELRDEGK#ASSAK 528
2264.7 219-233 LSQRFPK#AEFAEVSK 528
1995.5 337-348 RH#PDYSVVLLLR 528
1719.2 277-286 EC#C#EK#PLLEK 528
1404.5 74-81 LC#*TVATLR 528
1420.5 LC#*TVATLR 544
1353.6 535-541 H#K#PK#ATK 544
1014.2 1-4 DAH#K 544
1037.4 535-538 H#K#PK 528
2599.3 145-160 RH#PYFYAPELLFFAK#R 544
(a) Presumed modification sites of peptides analyzed by MALDI-TOF-MS are
in bold. Modification sites identified by ESI MS-MS are underlined.
Note: Presumed modification sites of peptides analyzed by MALDI-TOF-MS
are indicated with #. Modification sites identified by ESI MS-MS are
indicated with *.
Table 2. Tryptic peptides from serum albumin of a patient exposed to S.
chartarum.
m/z Amino acids Sequence (a) Adduct
1067.4 435-438 YTK#K 528
1109.4 464-468 H#PEAK 528
1226.2 29-34 SEVAH#R 528
1275.2 215-221 ASSAK#QR 528
1418.4 222-229 LK#C#ASLQK 528
1544.9 89-97 SLH#TLFGDK 528
1720.3 301-310 EC#C#EK#PLLEK 528
2911.1 76-97 TC#VADESAENC#DK#SLH#TLFGDK 528
1053.4 559-562 H#K#PK 544
1564.0 234-242 AFK#AWAVAR 544
2035.2 550-562 QTALVELVK#HK#PK 544
3910.1 37-65 DLGEENFK#ALVLIAFAQYLQQC#PEEDH#VK 544
(a) Amino acid residues that may be modified within the peptide are in
bold.
Note: Amino acid residues that may be modified within the peptide are
indicated with #.
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