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Dive into the research topics where Horacio Merchant is active.

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Featured researches published by Horacio Merchant.


Developmental Biology | 1975

Rat gonadal and ovarian organogenesis with and without germ cells. An ultrastructural study

Horacio Merchant

Abstract Busulphan (1, 4-butanediol dimetanosulfonate) a drug which selectively destroys primordial germ cells (PGC) was used to study its effects on the morphogenesis of the rat gonads. Undifferentiated gonads and ovaries taken daily from day 11 to birth were studied employing high resolution light and electron microscopy techniques. In these conditions it was established that PGC can be eliminated before arriving at the genital ridge when the drug is administered on the 11 day post coital. The absence of PGC does not prevent the initial proliferation of the somatic cells of the genital region. The morphogenetic events leading to the formation of an undifferentiated gonad, early sex differentiation and the establishment of an ovary are the same in sterilized and untreated embryos. Rat gonadal primordium developes from a blastema formed by proliferation of mesothelial and mesenchymal cells. The basal lamina of some mesonephric tubules is broken on one side and makes continuity with the forming basal lamina of the mesothelium of the genital ridge. In earlier stages mesonephric cells seem to freely mix with the other cells. From the blastema gradually emerges an epithelial tissue enveloped by a common basal lamina which includes the surface epithelium, epithelial “cords” and some mesonephric tubules. Early sex differentiation was determined by the precocious separation of the two latter tissues from the former in male embryos. In ovaries this epithelial tissue with or without germ cells maintains its identity the whole gestational life.


Archives of Andrology | 1982

Heparin Binding Sites in the Human Spermatozoa Membrane

N. M. Delgado; R. Reyes; L. Huacuja; Horacio Merchant; A. Rosado

The existence in the human spermatozoa membrane of receptorlike functional group for heparin was studied. Incubation of whole spermatozoa with tritiated heparin induced the specific binding of 745 +/- 112 pmol of heparin per 5 x 10(7) sperm cells with an intrinsic association constant KD = 3.6 x 10(-6) M. The specificity of binding was shown by the lack of competence in the binding process of some other glycosaminoglycans used at concentrations 20 x higher than heparin. However, dextran sulfate was a very efficient competitive agent. Autoradiography experiments showed that labeling was almost completely restricted to sperm cells in the process of nuclear decondensation. This technique showed the presence of a high amount of radioactive heparin in the isolated sperm membranes even after several washings. Heparin may participate both in the final part of the capacitation process (acrosome reaction) and in the decondensation of sperm nuclei.


Archives of Andrology | 1984

Glycosamineglycan sulfate as acrosomal reaction-inducing factor of follicular fluid.

R. Reyes; A. Carranco; Omar Hernández; A. Rosado; Horacio Merchant; N. M. Delgado

Follicular fluid from different mammalian species possesses two factors responsible for the induction of capacitation: a sperm-stimulating factor and an acrosomal reaction-inducing factor. The glycosamineglycan-sulfate (GAGs) extracted from pig follicular fluid induce acrosome reaction in pig spermatozoa which exhibit no morphological difference between the GAGs-induced reaction and the natural one. Acrosomal reaction commenced 30 min after the addition of GAGs and depended on GAGs concentration reaching 80% of acrosomal reacted spermatozoa after 6 hr of incubation with 7 mg of GAGs/ml. Chemical composition differs with the chemical data that characterize them as proteoglycans since those we obtained were practically protein free (2%). Another difference resides in the uronic acid content, which is almost twofold higher (59%). Electron microscope observations of the acrosomal reacted spermatozoa revealed that the addition of 10 mg/ml of trypsin soybean inhibitor did not interfere with any of the acrosomal reaction steps. The active capacitating factors may also originate from the follicular fluid released into the genital tract during ovulation.


Cancer Immunology, Immunotherapy | 2000

A recombinant vaccinia virus containing the papilloma E2 protein promotes tumor regression by stimulating macrophage antibody-dependent cytotoxicity

Carlos Rosales; Viviana Valadez Graham; Gerardo Arrellín Rosas; Horacio Merchant; Ricardo Rosales

Abstract Human papillomavirus infection is associated with cervical cancer. The E6 and E7 papillomavirus proteins are normally required for the maintenance of the malignant phenotype. Expression of these proteins in infected cells is negatively regulated by the binding of the papilloma E2 protein to the long terminal control region of the papilloma virus genome. The E2 protein can also promote cell arrest and apoptosis in HeLa cells. Therefore, it is clear that this protein has the potential of inhibiting the malignant phenotype. Because, anticancer vaccines based in vaccinia viruses have recently been shown to be an effective way to treat and to eradicate tumors, a recombinant vaccinia virus expressing the E2 gene of bovine papilloma virus (Modified Vaccinia Ankara, MVA E2) was created, to explore further the antitumor potential of the E2 protein. A series of rabbits, containing the VX2 transplantable papilloma carcinoma, were treated with MVA E2. An impressive tumor regression, up to a complete disappearance of tumor, was observed in most animals (80%). In contrast, very little or no regression was detected if the normal vaccinia virus was used. Lymphocytes isolated from MVA E2-treated rabbits did not show cytotoxic activity against tumor cells. However, in these animals a humoral immune response against tumor cells was observed. These antitumor antibodies were capable of activating macrophages to destroy tumor cells efficiently. These data indicate that injecting the MVA E2 recombinant vaccinia virus directly into the tumor results in a robust and long-lasting tumor regression. Data also suggest that antitumor antibodies are responsible, at least in part, for eliminating tumors by activating macrophage antibody-dependent cytotoxicity.


Biotechnology and Bioengineering | 2001

Comparative characterization of cell death between Sf9 insect cells and hybridoma cultures

Angélica Meneses-Acosta; Ronaldo Z. Mendonça; Horacio Merchant; Luis Covarrubias; Octavio T. Ramírez

Physiological cell death (PCD) in Sf9 insect cell batch cultures was comprehensively characterized using simultaneous determinations of qualitative and quantitative assays, including agarose gel electrophoresis, confocal, epifluorescence, and transmission electron microscopy, and DNA content by flow cytometry. Results were compared to hybridoma cultures where abundant information of apoptosis exists. Both cultures shared some typical apoptosis features, including cell shrinkage, loss of sphericity, swollen endoplasmic reticulum and Golgi apparatus, chromatin condensation, and specific DNA degradation. However, distinctive morphological and kinetic differences between both cultures revealed that Sf9 cells died by an atypical PCD process characterized by absence of nuclear fragmentation, scarce association of condensed chromatin to the nuclear envelope, swollen mitochondria, and high nonspecific DNA degradation. These features, distinctive of necrosis, were not observed in the normal apoptotic process of hybridomas. Glucose depletion marked the appearance of apoptotic Sf9 cells, which there up on increased gradually, whereas apoptotic hybridomas rapidly increased upon glutamine depletion. Furthermore, active phagocytosis was found in Sf9 viable cells, a characteristic phenomenon during in vivo apoptosis but uncommon for in vitro cultures. Sf9 cells contained unusually high numbers of phagosomes, particularly after glucose depletion. Additionally, few apoptotic bodies accumulated in culture, suggesting their elimination by phagocytosis. Other distinctive characteristics of Sf9 cells were the presence of a polynucleated hypertrophic population fraction, polyploidy, cell cycle arrest in G2/M phase, and more necrosis compared to hybridomas. Such phenomena prevented a reliable quantification of apoptosis from determination of the sub-G1 peak. Nonetheless, emergence of a bimodal Sf9 cell size distribution coincided with the increase in the sub-G1 population and onset of death. The fraction of particles in the smaller peak (6-11 microm diameter) closely correlated with the fractions of apoptotic bodies, late apoptotic, and secondary necrotic cells. Accordingly, Sf9 cell size was shown to be an effective, rapid, and simple parameter for quantifying death. Altogether, the results of this study provide new insights into PCD and other phenomena in insect cell culture important for biotechnological applications of Sf9 cells.


Archives of Andrology | 1983

Heparin-Induced Nuclei Decondensation of Mammalian Epididymal Spermatozoa

A. Carranco; R. Reyes; V. M. Magdaleno; L. Huacuja; O. Hernández; A. Rosado; Horacio Merchant; N. M. Delgado

Decondensation of mammalian epididymal spermatozoa nuclei has been induced by exposure of intact spermatozoa to heparin, including those species in which ejaculated sperm were not susceptible to this treatment. This process occurred in the absence of any disulfide bond cleaving reactant. Swelling of caput epididymal spermatozoa nuclei commenced about 30 min after the addition of heparin, reaching 88% in rat, 33% in rabbit, 26% in pig, and 62% in bull of swelled nuclei after 6 hr of incubation at 37 degrees C with 5000 USP of heparin per ml. Corpus epididymal spermatozoa nuclei of rat and rabbit underwent decondensation at 50 degrees C reaching 24% and 22% of swelled nuclei, respectively, after 6 hr of incubation. The nuclei of the sperm cells of pig and bull from this epididymal region remained highly condensed as well as the nuclei of the cauda epididymal spermatozoa of all the species assayed. Electron microscope observations of the caput epididymal spermatozoa nuclei treated with heparin revealed that the chromatin is organized into nuclear bodies joined by a network of cross-linked and branched chromatin fibers in the species studied.


Cancer | 2000

Human Tumor Growth Is Inhibited by a Vaccinia Virus Carrying the E2 Gene of Bovine Papillomavirus

Viviana Valadez Graham; Gerd Sutter; Marco V. José; Alejandro García-Carranca; Volker Erfle; Norma Moreno Mendoza; Horacio Merchant; Ricardo Rosales

Papillomavirus is the etiologic agent associated with cervical carcinoma. The papilloma E2 protein is able to regulate negatively the expression of E6 and E7 papilloma oncoproteins. Therefore, a new, highly attenuated vaccinia virus known as modified vaccinia virus Ankara (MVA), which carries the papillomavirus E2 gene, was used for the treatment of tumors associated with human papillomavirus.


Journal of the Neurological Sciences | 2007

Functional and morphological effects of repeated sodium arsenite exposure on rat peripheral sensory nerves

Erika García-Chávez; Bertha Segura; Horacio Merchant; Ismael Jiménez; Luz M. Del Razo

Exposure to inorganic arsenic (iAs) is known to result in peripheral neuropathy. To better understand the functional and morphological consequences of iAs exposure, we examined the electrophysiological and histological characteristics of the sensory sural nerves in adult Male Wistar rats following 30 days of sodium arsenite administration by gavage (10 mg/kg body weight/day). Arsenic (As) levels in the peripheral nerves of exposed animals were about 150 times greater than those in controls. Lipid peroxidation was also increased in iAs-exposed animals. Compound action potentials (CAPs) evoked in iAs-exposed nerves were characterized by a slower conduction velocity ( approximately 26%). iAs-exposed nerves also showed a trend towards a decreased CAP area ( approximately 35%). These electrophysiological changes were consistent with histological alterations such as a approximately 56% decrease in myelin thickness. In addition, the perimeter and transverse area of axons were reduced to 29% and 45% of control, respectively. Our results suggest that accumulation of As produced by iAs exposure induces oxidative damage, severe demyelination, and other morphological alterations in axons of peripheral nerves. These changes may, in turn, induce changes in the generation and propagation of action potentials in peripheral nerves, leading to decreased transmission of information from peripheral sensory organs to the central nervous system.


Archives of Andrology | 1984

Heparin-induced release of DNA template restrictions in human sperm zinc-depleted nuclei.

N. M. Delgado; V. M. Magdaleno; Horacio Merchant; A. Rosado; R. Reyes

The addition of heparin to human sperm zinc-depleted nuclei releases DNA template restrictions. Spermatozoa depleted of zinc were assayed for (3H-methyl), thymidine incorporation was observed (27,500 +/- 1,248 dpm of 3H methyl-thymidine). Sperm cells incubated in the presence of 10 mg/ml of soybean trypsin inhibitor shows no effect in sperm nuclear swelling or in the release of DNA template restrictions. This process runs in a parallel fashion to the nuclear swelling induced by heparin, suggesting that swollen nuclei might be the source of DNA template. This was confirmed by autoradiographic studies, since all the sperm cells whose nuclei were judged swollen by morphological criteria also appeared labeled. The fact that there was no need for ATP generating system or of exogenous DNA polymerase emphasized the control role that zinc plays in the physiology of the human spermatozoa.


Fertility and Sterility | 1976

Changes in the Protein Conformation of Human Spermatozoal Membranes after Treatment with Cyclic Adenosine 3′ :5′ -Monophosphate and Human Follicular Fluid

Néstor M. Delgado; Luis Huacuja; Rosa Ma. Pancardo; Horacio Merchant; Adolfo Rosado

Infrared spectra in the amide I and amide II regions of acrosomal membranes isolated from ejaculated human spermatozoa indicate the presence of a high proportion of the constitutive proteins in the most stable protein configuration, the antiparallel beta-conformation. Since the infrared spectra obtained with the membranes suspended in D2O or after extraction of the lipid components do not show any significant change, it can be postulated that the antiparallel pleated sheet conformation of human spermatozoal membrane proteins is independent of the hydrated state and of the lipid constitution of the membrane.

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N. M. Delgado

Mexican Social Security Institute

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R. Reyes

Mexican Social Security Institute

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A. Rosado

Universidad Autónoma Metropolitana

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L. Huacuja

Mexican Social Security Institute

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A. Carranco

Mexican Social Security Institute

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Adolfo Rosado

Mexican Social Security Institute

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Angélica Meneses-Acosta

Universidad Autónoma del Estado de Morelos

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Bertha Segura

National Autonomous University of Mexico

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Ricardo Rosales

National Autonomous University of Mexico

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