Your search keyword '"Serum -- Research"' showing total 11 results

1. Distinct roles of haptoglobin-related protein and apolipoprotein L-I in trypanolysis by human serum

Author

Vanhollebeke, Benoit, Nielsen, Marianne J., Watanabe, Yoshihisa, Truc, Philippe, Vanhamme, Luc, Nakajima, Kazunori, Moestrup, Soren K., and Pays, Etienne

Subjects

Haptoglobin -- Research, Apolipoproteins -- Research, Serum -- Research, Trypanosoma brucei -- Research, Science and technology

Abstract

Apolipoprotein L-I (apoL-I) is a human high-density lipoprotein (HDL) component able to kill Trypanosorna brucei brucei by forming anion-selective pores in the lysosomal membrane of the parasite. Another HDL component, haptoglobin-related protein (Hpr), has been suggested as an additional toxin required for full trypanolytic activity of normal human serum. We recently reported the case of a human lacking apoL-I ([apoL-I.sup.-/-]HS) as the result of frameshift mutations in both apoL-I alleles. Here, we show that this serum, devoid of any trypanolytic activity, exhibits normal concentrations of HDL-bound Hpr. Conversely, the serum of individuals with normal HDL-bound apoL-I but who lack Hpr and haptoglobin [[Hp(r).sup.-/-]HS] as the result of gene deletion (anhaptoglobinemia) exhibited phenotypically normal but delayed trypanolytic activity. The trypanolytic properties of [Hp(r).sup.-/-]HS were mimicked by free recombinant apoL-I, whereas recombinant Hpr did not affect trypanosomes. The lysis delay observed with either [Hp(r).sup.-/-]HS or recombinant apoL-I could entirely be attributed to a defect in the uptake of the lytic components. Thus, apoL-I is responsible for the trypanolytic activity of normal human serum, whereas Hpr allows fast uptake of the carrier HDL particles, presumably through their binding to an Hp/Hpr surface receptor of the parasite. innate immunity | sleeping sickness | rypanolytic factor | haptoglobin receptor | Trypanosoma brucei

Published

2007

2. Decreased levels of CXC-chemokines in serum of benzene-exposed workers identified by array-based proteomics

Author

Vermeulen, Roel, Lan, Qing, Zhang, Luoping, Gunn, Laura, McCarthy, Diane, Woodbury, Ronald L., McGuire, Marielena, Podust, Vladimir N., Li, Guilan, Chatterjee, Nilanjan, Mu, Ruidong, Yin, Songnian, Rothman, Nathaniel, and Smith, Martyn T.

Subjects

Benzene -- Chemical properties, Benzene -- Contamination, Leukemia -- Causes of, Leukemia -- Research, Serum -- Research, Science and technology

Abstract

Benzene is an important industrial chemical and environmental contaminant that causes leukemia. To obtain mechanistic insight into benzene's mechanism of action, we examined the impact of benzene on the human serum proteome in a study of exposed healthy shoe-factory workers and unexposed controls. Two sequential studies were performed, each using sera from 10 workers exposed to benzene (overall mean benzene air level >30 ppm) and 10 controls. Serum samples were subjected to anion-exchange fractionation and bound to three types of ProteinChip arrays (Ciphergen Biosystems, Fremont, CA) [hydrophobic (H50), metal affinity (IMAC3-Cu), and cation exchange (WCX2)]. Protein-expression patterns were detected by surface-enhanced laser desorption/ ionization (SELDI)-TOF MS. Three proteins (4.1, 7.7, and 9.3 kDa) were consistently down-regulated in exposed compared with control subjects in both studies. All proteins were highly inversely correlated with individual estimates of benzene exposure (r > 0.75). The 7.7- and 9.3-kDa proteins were subsequently identified as platelet factor (PF)4 and connective tissue activating peptide (CTAP)-III. Initial proteomic results for PF4 and CTAP-III were subsequently confirmed in a single experiment using a Protein-Chip-array-based immunoassay(Ciphergen Biosystems). The altered expression of the platelet-derived CXC-chemokines (40% and 63% for PF4 and CTAP-III, respectively) could not be explained by changes in absolute platelet counts. Thus, SELDI-TOF analysis of a limited number of exposed and unexposed subjects revealed that lowered expression of PF4 and CTAP-III proteins is a potential biomarker of benzene's early biologic effects and may play a role in the immunosuppressive effects of benzene. biomarker | leukemia | mass spectrometry | platelet | molecular epidemiology

Published

2005

3. Ribonuclease A variants with potent cytotoxic activity

Author

Leland, Peter A., Schultz, L. Wayne, Kim, Byung-Moon, and Raines, Ronald T.

Subjects

Ribonuclease -- Research, Serum -- Research, Catalysis -- Research, Science and technology

Abstract

Select members of the bovine pancreatic ribonuclease A (RNase A) superfamily are potent cytotoxins. These cytotoxic ribonucleases enter the cytosol, where they degrade cellular RNA and cause cell death. Ribonuclease inhibitor (RI), a cytosolic protein, binds to members of the RNase A superfamily with inhibition constants that span 10 orders of magnitude. Here, we show that the affinity of a ribonuclease for RI plays an integral role in defining the potency of a cytotoxic ribonuclease. RNase A is not cytotoxic and binds RI with high affinity. Onconase, a cytotoxic RNase A homolog, binds RI with low affinity. To disrupt the RI-RNase A interaction, three RNase A residues (Asp-38, Gly-88, and Ala-109) that form multiple contacts with RI were replaced with arginine. Replacing Asp-38 and Ala-109 with an arginine residue has no effect on the RI-RNase interaction. In addition, these variants are not cytotoxic. In contrast, replacing Gly-88 with an arginine residue yields a ribonuclease (G88R RNase A) that retains catalytic activity in the presence of R1 and is cytotoxic to a transformed cell line. Replacing Gly-88 with aspartate also yields a ribonuclease (G88D RNase A) with a decreased affinity for RI and cytotoxic activity. The cytotoxic potency of onconase, G88R RNase A, and G88D RNase A correlate with RI evasion. We conclude that ribonucleases that retain catalytic activity in the presence of RI are cytotoxins. This finding portends the development of a class of chemotherapeutic agents based on pancreatic ribonucleases.

Published

1998

4. Vitamin A in serum is a survival factor for fibroblasts

Author

Chen, Yanqui, Derguini, Fadila, and Buck, Jochen

Subjects

Vitamin A -- Research, Fibroblasts -- Analysis, Serum -- Research, Science and technology

Abstract

Murine 3T3 cells arrest in a quiescent, nondividing state when transferred into medium containing little or no serum. Within the first day after transfer, fibroblasts can be activated to proliferate by platelet-derived growth factor (PDGF) alone; cells starved longer than 1 day, however, are activated only by serum. We demonstrate that endogenous vitamin A (retinol) or retinol supplied by serum prevents cell death and that retinol, in combination with PDGF, can fully replace serum in activating cells starved longer than 1 day. The physiological retinol derivative 14-hydroxy-4,14-retro-retinol, but not retinoic acid, can replace retinol in rescuing or activating 3T3 cells. Anhydroretinol, another physiological retinol metabolite that acts as a competitive antagonist of retinol, blocks cell activation by serum, indicating that retinol is a necessary component of serum. It previously has been proposed that activation of 3T3 cells requires two factors in serum, an activation factor shown to be PDGF and an unidentified survival factor. We report that retinol is the survival factor in serum.

Published

1997

5. A diffusable cytotoxin of Haemophilus ducreyi

Author

Cope, Leslie D., Lumbley, Sheryl, Latimer, Jo L., Klesney-Tait, Julia, Stevens, Marla K., Johnson, Linda S., Purven, Maria, Munson, Robert S., Jr., Lagergard, Teresa, Radolf, Justin D., and Hansen, Eric J.

Subjects

Hemophilus infections -- Research, Serum -- Research, Ulcers -- Microbiology, Science and technology

Abstract

Little is known about the virulence mechanisms employed by Haemophilus ducreyi in the production of genital ulcers. This Gram-negative bacterium previously has been shown to produce a soluble cytotoxic activity that kills HeLa and HEp-2 cells. We have now identified a cluster of three H. ducreyi genes that encode this cytotoxic activity. The predicted proteins encoded by these genes are most similar to the products of the Escherichia coli cdtABC genes that comprise the cytolethal distending toxin (CDT) of this enteric pathogen. Eleven of 12 H. ducreyi strains were shown to possess this gene cluster and culture supernatants from these strains readily killed HeLa cells. The culture supernatant from a single strain of H. ducreyi that lacked these genes was unable to kill HeLa cells. When the H. ducreyi cdtABC gene cluster was cloned into E. coli, culture supernatant from the recombinant E. coli clone killed HeLa cells. A monoclonal antibody that neutralized this soluble cytotoxic activity of H. ducreyi was shown to bind to the H. ducreyi cdtC gene product. This soluble H. ducreyi cytotoxin may play a role in the development or persistence of the ulcerative lesions characteristic of chancroid.

Published

1997

6. Multidrug resistance mediated by a bacterial homolog of the human multidrug transporter MDR1

Author

Veen, Hendrik W. van, Kenema, Koen, Bolhuis, Henk, Oussenko, Irina, Kok, Jan, Poolman, Bert, Driessen, Arnold J.M., and Konings, Wil N.

Subjects

Drug resistance in microorganisms -- Genetic aspects, Serum -- Research, Cloning -- Research, Science and technology

Abstract

Resistance of Lactococcus lactis to cytotoxic compounds shares features with the multidrug resistance phenotype of mammalian tumor cells. Here, we report the gene cloning and functional characterization in Escherichia coli of LmrA, a lactococcal structural and functional homolog of the human multidrug resistance P-glycoprotein MDR1. LmrA is a 590-aa polypeptide that has a putative topology of six [Alpha]-helical transmembrane segments in the N-terminal hydrophobic domain, followed by a hydrophilic domain containing the ATP-binding site. LmrA is similar to each of the two halves of MDR1 and may function as a homodimer. The sequence conservation between LmrA and MDR1 includes particular regions in the transmembrane domains and connecting loops, which, in MDR1 and the MDR1 homologs in other mammalian species, have been implicated as determinants of drug recognition and binding. LmrA and MDR1 extrude a similar spectrum of amphiphilic cationic compounds, and the activity of both systems is reversed by reserpine and verapamil. As LmrA can be functionally expressed in E. coli, it offers a useful prokaryotic model for future studies on the molecular mechanism of MDR1-like multidrug transporters.

Published

1996

7. Delineation of the subunit composition of human proteasomes using antisera against the major histocompatibility complex-encoded LMP2 and LMP7 subunits

Author

Patel, Salil D., Monaco, John J., and McDevitt, Hugh O.

Subjects

Histocompatibility -- Research, Serum -- Research, Proteases -- Research, Antibodies -- Research, Science and technology

Abstract

A sequential analysis using antibodies revealed two human proteasome subunits, related to the major histocompatibility complex-encoded LMP2 and LMP7. LMP2 occurs in two forms, unprocessed and processed forms. Anti-LMP2 serum releases a proteasome-ike complex which contains one LMP2 isoform and lacks LMP7. The serum structure has four novel subunits, including LMP2A which is a proteasome precursor.

Published

1994

8. Epithelial autotoxicity of nitric oxide: role in the respiratory cytopathology of pertussis

Author

Heiss, Linda Nixon, Lancaster, Jack R. , Jr., Corbett, John A., and Goldman, William E.

Subjects

Bordetella pertussis -- Research, Epithelial cells -- Research, Interleukin-1 -- Research, Serum -- Research, Science and technology

Abstract

An analysis of Bordetella pertussis epithelial cells reveals that the tracheal cytotoxin (TCT)-cytokine, interleukin (IL-1), depends on nitric oxide synthesis to attack target cells. Respiratory epithelial cells generate nitric oxide on exposure to TCT and also generate IL-1. TCT is the virulence factor that duplicates pertussis and respiratory cytopathology.

Published

1994

9. Stability of cytotoxic luteinizing hormone-releasing hormone conjugate (AN-152) containing doxorubicin 14-O-hemiglutarate in mouse and human serum in vitro: Implications for the design of preclinical studies

Author

Nagy, Attila, Plonowski, Artur, and Schally, Andrew V.

Subjects

Serum -- Research, Peptides -- Research, Nude mouse -- Research, Chemotherapy -- Research, Science and technology

Abstract

Recently, we developed a series of cytotoxic peptide conjugates containing 14-O-glutaryl esters of doxorubicin (DOX) or 2-pyrrolino-DOX (AN-201). Serum carboxylesterase enzymes (CE) can partially hydrolyze these conjugates in the circulation, releasing the cytotoxic radical, before the targeting is complete. CE activity in serum of nude mice is about 10 times higher than in human serum. Thus, we found that the [t.sub.1/2] of AN-152, an analog of luteinizing hormone-releasing hormone (LH-RH) containing DOX, at 0.3 mg/ml is 19.49 [+ or -] 0.74 min in mouse serum and 126.06 [+ or -] 3.03 min in human serum in vitro. The addition of a CE inhibitor, diisopropyl fluorophosphate (DFP), to mouse serum in vitro significantly (P [is less than] 0.01) prolongs the [t.sub.1/2] of AN-152 to 69.63 [+ or -] 4.44 min. When DFP is used in vivo, 400 nmol/kg cytotoxic somatostatin analog AN-238 containing AN-201 is well tolerated by mice, whereas all animals die after the same dose without DFP. In contrast, DFP has no effect on the tolerance of AN-201. A better tolerance to AN-238 after DFP treatment is due to the selective uptake of AN-238 by somatostatin receptor-positive tissues. Our results demonstrate that the suppression of the CE activity in nude mice greatly decreases the toxicity of cytotoxic hybrids containing 2-pyrrolino-DOX 14-O-hemiglutarate and brings this animal model closer to the conditions that exist in humans. The use of DFP together with these peptide conjugates in nude mice permits a better understanding of their mechanism of action and improves the clinical predictability of the oncological and toxicological results. targeted chemotherapeutic agents | tolerance | esterase inhibitors | diisopropyl fluorophosphate

Published

2000

10. Double trans-chromosomic mice: Maintenance of two individual human chromosome fragments containing Ig heavy and [Kappa] loci and expression of fully human antibodies

Author

Tomizuka, Kazuma, Shinohara, Tokuyuki, Yoshida, Hitoshi, Uejima, Hiroshi, Ohguma, Atsuko, Tanaka, Sonoko, Sato, Kaoru, Oshimura, Mitsuo, and Ishida, Isao

Subjects

Human chromosomes -- Research, Mice -- Physiological aspects, Serum -- Research, Immunization -- Analysis, Science and technology

Abstract

The use of a human chromosome or its fragment as a vector for animal transgenesis may facilitate functional studies of large human genomic regions. We describe here the generation and analysis of double trans-chromosomic (Tc) mice harboring two individual human chromosome fragments (hCFs). Two transmittable hCFs, one containing the Ig heavy chain locus (IgH, [approximately equals] 1.5 Mb) and the other the K light chain locus (Ig[Kappa], [approximately equals]2 Mb), were introduced into a mouse strain whose endogenous IgH and Ig[Kappa] loci were inactivated. In the resultant double-Tc/double-knockout mice, substantial proportion of the somatic cells retained both hCFs, and the rescue in the defect of Ig production was shown by high level expression of human Ig heavy and K chains in the absence of mouse heavy and [Kappa] chains. In addition, serum expression profiles of four human Ig [Gamma] subclasses resembled those seen in humans. They mounted an antigen-specific human antibody response upon immunization with human serum albumin, and human serum albumin-specific human monoclonal antibodies with various isotypes were obtained from them. These results represent a generation of mice with 'humanized' loci by using the transmittable hCFs, which suggest that the Tc technology may allow for the humanization of over megabase-sized, complex loci in mice or other animals. Such animals may be useful not only for studying in vivo functions of the human genome but also for obtaining various therapeutic products.

Published

2000

11. Oncogenic stimulation recruits cyclin-dependent kinase in the cell cycle start in rat fibroblast

Author

Jinno, Shigeki, Hung, Shih-Chieh, Yamamoto, Hanako, Lin, Jie, Nagata, Akihisa, and Okayama, Hiroto

Subjects

Cells -- Analysis, Serum -- Research, Oncogenes -- Research, Growth -- Analysis, Cell cycle -- Research, Science and technology

Abstract

The rat fibroblast NRK cells are transformed reversibly by a combination of growth factors. When stimulated with serum, NRK cells rely on cyclin-dependent kinase 4 (Cdk4) for their S phase entry. However, when stimulated with serum containing oncogenic growth factors, they come to rely on either Cdk4 or Cdk6, and their S phase entry cannot be blocked unless both Cdk4 and Cdk6 are immunodepleted. Such change of dependence does not occur in the NRK cell mutants defective in an oncogenic signal pathway and, therefore, deficient in anchorage-independent cell cycle start ability, correlating Cdk6 dependence with this remarkable, cancer-associated phenotype. However, both Cdk4 and Cdk6 are activated upon serum stimulation, and neither the amounts of Cdk6, Cdk4, cyclin D1, and cyclin-dependent kinase inhibitors nor the activities or subcellular localization of Cdk6 and Cdk4 are significantly influenced by oncogenic stimulation. Thus, oncogenic stimulation invokes Cdk6 to participate in a critical step of the cell cycle start in a rat fibroblast, but by a mechanism seemingly unrelated to the regulation of the kinase. Given that many hematopoietic cells employ predominantly Cdk6 for the cell cycle start and perform anchorage-independent growth by nature, our results raise the possibility that the oncogenic stimulation-induced anchorage-independent cell cycle start of NRK is elicited by a mechanism similar to the one used for hematopoietic cell proliferation. NRK | [G.sub.1] | Cdk4 | transformation

Published

1999