Your search keyword '"Shin Hyeong Cho"' showing total 222 results

201. Molecular Cloning of Plasmodium vivax Calcium-Dependent Protein Kinase 4.

Author

Kyung-Mi Choi, Jung-Yeon Kim, Sung-Ung Moon, Hyeong-Woo Lee, Sattabongkot, Jetsumon, Byoung-Kuk Na, Dae-Won Kim, Eun-Jung Suh, Yeon-Joo Kim, Shin-Hyeong Cho, Ho-Sa Lee, Ho-Gun Rhie, and Tong-Soo Kim

Subjects

PLANTS, MOLECULAR cloning, PLASMODIUM vivax, CALCIUM, PROTEIN kinases, ENZYMES, ESCHERICHIA coli

Published

2010

202. Prevalence of Toxoplasma gondii Infection in Stray and Household Cats in Regions of Seoul, Korea.

Author

Sang-Eun Lee, Jae-Yeong Kim, Yun-Ah Kim, Shin-Hyeong Cho, Hye-Jin Ahn, Heung-Myong Woo, Won-Ja Lee, and Ho-Woo Nam

Subjects

VETERINARY protozoology, TOXOPLASMA gondii, CAT diseases, IMMUNOGLOBULINS, ENZYME-linked immunosorbent assay, POLYMERASE chain reaction

Published

2010

203. Proteomic Analysis of Haptoglobin and Amyloid A Protein Levels in Patients with Vivax Malaria.

Author

Young Yil Bahk, Byoung-Kuk Na, Shin-Hyeong Cho, Jung-Yeon Kim, Kook-Jin Lim, and Tong-Soo Kim

Subjects

PROTEOMICS, HAPTOGLOBINS, AMYLOID, GLYCOPROTEINS, MALARIA treatment, PLASMODIUM vivax, MASS spectrometry, TWO-dimensional electrophoresis

Published

2010

204. Epidemiological Survey on the Infection of Intestinal Flukes in Residents of Muan-gun, Jeollanam-do, the Republic of Korea.

Author

Shin-Hyeong Cho, Pyo-Yun Cho, Dong-Min Lee, Tong-Soo Kim, In-Sang Kim, Eun-Jung Hwang, Byoung-Kuk Na, and Woon-Mok Sohn

Subjects

INFECTION, HELMINTHS, WORM eggs, MICROBIOLOGY, FECES

Abstract

Infection status of intestinal flukes was investigated in residents of Muan-gun, Jeollanam-do, the Republic of Korea. Total 1,257 fecal samples of residents were examined by formalin-ether sedimentation technique and Kato-Katz thick smear method. Helminth eggs were detected from 95 (7.6%) residents, and eggs of heterophyid flukes and Clonorchis sinensis were found from 62 (4.9%) and 40 (3.2%) cases, respectively. The larger heterophyid eggs, somewhat dark-brown in color and 37.7 x 21.5 mm in average size, and found in 32 (2.6%) out of 62 egg positive cases of heterophyid flukes. To confirm the adult flukes, we performed worm recovery from 12 cases after praziquantel treatment and purgation with MgSO4. A total of 1,281 adult flukes, assigned to 7 species, were recovered from 9 cooperative cases. Heterophyes nocens (total 981 specimens) was collected from 9 cases, Stictodora fuscata (80) from 7, Gymnophalloides seoi (75) from 5, Pygidiopsis summa (140) from 3, Stellantchasmus falcatus (3) from 2, and Stictodora lari and Acanthotrema felis (each 1 worm) from 1 case each. The intrauterine eggs of S. fuscata collected from the recovered worm were identical with the larger heterophyid eggs detected in the stool examination. By the present study, it was confirmed that A. felis is a new intestinal fluke infecting humans, and residents in Muan-gun, Jeollanam-do are infected with variable species of intestinal trematodes. [ABSTRACT FROM AUTHOR]

Published

2010

205. Infection Status of Hospitalized Diarrheal Patients with Gastrointestinal Protozoa, Bacteria, and Viruses in the Republic of Korea.

Author

Hyeng-Il Cheun, Shin-Hyeong Cho, Jin-Hee Lee, Yi-Young Lim, Ji-Hye Jeon, Jae-Ran Yu, Tong-Soo Kim, Won-Ja Lee, Seung-Hak Cho, Deog-Yong Lee, Mi-Seon Park, Hye-Sook Jeong, Doo-Sung Chen, Yeong-Mi Ji, and Mi-Hwa Kwon

Subjects

PROTOZOA, VIRUS diseases, BACTERIAL diseases, DIARRHEA, CRYPTOSPORIDIUM parvum, ENTAMOEBA histolytica

Abstract

To understand protozoan, viral, and bacterial infections in diarrheal patients, we analyzed positivity and mixed-infection status with 3 protozoans, 4 viruses, and 10 bacteria in hospitalized diarrheal patients during 2004-2006 in the Republic of Korea. A total of 76,652 stool samples were collected from 96 hospitals across the nation. The positivity for protozoa, viruses, and bacteria was 129, 1,759, and 1,797 per 10,000 persons, respectively. Especially, Cryptosporidium parvum was highly mixed-infected with rotavirus among pediatric diarrheal patients (29.5 per 100 C. parvum positive cases), and Entamoeba histolytica was mixed-infected with Clostridium perfringens (10.3 per 100 E. histolytica positive cases) in protozoan-diarrheal patients. Those infected with rotavirus and C. perfringens constituted relatively high proportions among mixed infection cases from January to April. The positivity for rotavirus among viral infection for those aged ≤ 5 years was significantly higher, while C. perfringens among bacterial infection was higher for ≥ 50 years. The information for association of viral and bacterial infections with enteropathogenic protozoa in diarrheal patients may contribute to improvement of care for diarrhea as well as development of control strategies for diarrheal diseases in Korea. [ABSTRACT FROM AUTHOR]

Published

2010

206. Functional expression and characterization of a cytosolic copper/zinc-superoxide dismutase of Spirometra erinacei.

Author

Ai-Hua Li, Byoung-Kuk Na, Sung-Kyu Ahn, Shin-Hyeong Cho, Jhang-Ho Pak, Yun-Kyu Park, and Tong-Soo Kim

Subjects

SUPEROXIDE dismutase, PSEUDOPHYLLIDEA, INTESTINAL infections, MOLECULAR genetics, ENZYME analysis, HOST-parasite relationships, AMINO acid sequence

Abstract

Abstract   Spirometra erinacei is a pseudophyllidean tapeworm which inhabits the intestines of cats and dogs. The infections are usually asymptomatic in these animals, but the infection of the plerocercoid larvae of the parasite, spargana, cause sparganosis in other vertebrates, including human. In this study, we identified a gene encoding the copper/zinc-superoxide dismutase of S. erinacei (SeCuZnSOD) and partially characterized the biochemical and functional properties of the enzyme. The open reading frame of SeCuZnSOD was 465 bp that encodes 154 amino acids. The characteristic amino acid residues and motifs required for coordinating copper and zinc enzymatic function were well conserved. The genomic length of the SeCuZnSOD was 1,985 bp consisting of three exons that are separated by two introns. SeCuZnSOD is a typical cytosolic form which shares similar biochemical properties, including broad pH optima and inhibition profile by KCN and H2O2, with cytosolic Cu/Zn–SODs of other organisms. SeCuZnSOD was functionally expressed in both S. erinacei plerocercoid larvae and adult worms, and its expression level was significantly increased when the plerocercoid larvae were treated with paraquat. The enzyme may play essential roles for survival of the parasite not only by protecting itself from endogenous oxidative stress, but also by detoxifying oxidative killing of the parasite by host immune effector cells. [ABSTRACT FROM AUTHOR]

Published

2010

207. Prevalence of Plasmodium vivax VK210 and VK247 subtype in Myanmar.

Author

Tong-Soo Kim, Hyung-Hwan Kim, Sun-Sim Lee, Byoung-Kuk Na, Khin Lin, Shin-Hyeong Cho, Yoon-Joong Kang, Do-Kyung Kim, Youngjoo Sohn, Hyuck Kim, and Hyeong-Woo Lee

Subjects

PLASMODIUM vivax, AMINO acids, HUMAN chromosome abnormality diagnosis, POLYMERASE chain reaction

Abstract

Background: Plasmodium vivax is divided into two subtypes, a dominant form, VK210 and a variant form, VK247. This division is dependent on the amino acid composition of the circumsporozoite (CS) protein. In this study, the prevalence of the VK247 variant form of P. vivax was investigated in Myanmar. Methods: The existence of malaria parasites in blood samples was determined by microscopic examination, polymerase chain reaction (PCR) and DNA hybridization assays. To test for antibodies against P. vivax and Plasmodium falciparum in blood samples, an indirect immunofluorescence antibody test (IFAT) was performed using asexual blood antigens. An enzyme-linked immunosorbent assay with synthetic VK210 and VK247 antigens was carried out to discriminate between the P. vivax subtypes. Results: By thick smear examination, 73 (n = 100) patients were single infected with P. vivax, one with P. falciparum and 13 with both species. By thin smear, 53 patients were single infected with P. vivax, eight with only P. falciparum and 16 with both. Most of the collected blood samples were shown to be P. vivax positive (n = 95) by PCR. All cases that were positive for P. falciparum by PCR (n = 43) were also positive for P. vivax. However, 52 cases were single infected with P. vivax. IFAT showed antibody titres from 1:32 to 1:4,096. Additionally, using specific antibodies for VK210 and VK247, ELISA showed that 12 patients had antibodies for only the VK210 subtype, 4 patients had only VK247 subtype antibodies and 21 patients had antibodies for both subtypes. Using a DNA hybridization test, 47 patients were infected with the VK210 type, one patient was infected with VK247 and 23 patients were infected with both subtypes. Conclusions: The proportion of the VK247 subtype in Myanmar was 43.1% (n = 25) among 58 positive cases by serodiagnosis and 25.6% (n = 24) among 94 positive cases by genetic diagnosis. In both diagnostic methods, the infection status of malaria patients is highly diverse with respect to malaria species, and multiple clonal infections are prevalent in Myanmar. Therefore, the complexity of the infection should be considered carefully when diagnosing malaria in Myanmar. [ABSTRACT FROM AUTHOR]

Published

2010

208. Genetic polymorphism of merozoite surface protein-1 and merozoite surface protein-2 in Plasmodium falciparum field isolates from Myanmar.

Author

Jung-Mi Kang, Sung-Ung Moon, Jung-Yeon Kim, Shin-Hyeong Cho, Khin Lin, Woon-Mok Sohn, Tong-Soo Kim, and Byoung-Kuk Na

Subjects

GENETIC polymorphisms, MALARIA, PREVENTIVE medicine, IMMUNOGLOBULINS

Abstract

Background: Merozoite surface protein-1 (MSP-1) and MSP-2 of Plasmodium falciparum are potential vaccine candidate antigens for malaria vaccine development. However, extensive genetic polymorphism of the antigens in field isolates of P. falciparum represents a major obstacle for the development of an effective vaccine. In this study, genetic polymorphism of MSP-1 and MSP-2 among P. falciparum field isolates from Myanmar was analysed. Methods: A total of 63 P. falciparum infected blood samples, which were collected from patients attending a regional hospital in Mandalay Division, Myanmar, were used in this study. The regions flanking the highly polymorphic characters, block 2 for MSP-1 and block 3 for MSP-2, were genotyped by allele-specific nested-PCR to analyse the population diversity of the parasite. Sequence analysis of the polymorphic regions of MSP-1 and MSP-2 was also conducted to identify allelic diversity in the parasite population. Results: Diverse allelic polymorphism of MSP-1 and MSP-2 was identified in P. falciparum isolates from Myanmar and most of the infections were determined to be mixed infections. Sequence analysis of MSP-1 block 2 revealed that 14 different alleles for MSP-1 (5 for K1 type and 9 for MAD20 type) were identified. For MSP-2 block 3, a total of 22 alleles (7 for FC27 type and 15 for 3D7 type) were identified. Conclusion: Extensive genetic polymorphism with diverse allele types was identified in MSP-1 and MSP-2 in P. falciparum field isolates from Myanmar. A high level of mixed infections was also observed, as was a high degree of multiplicity of infection. [ABSTRACT FROM AUTHOR]

Published

2010

209. Successful Control of Lymphatic Filariasis in the Republic of Korea.

Author

Hyeng-Il Cheun, Yoon Kong, Shin-Hyeong Cho, Jong-Soo Lee, Jong-Yil Chai, Joo-Shil Lee, Jong-Koo Lee, and Tong-Soo Kim

Subjects

FILARIASIS prevention, LYMPHATIC diseases, ECONOMIC development, HYGIENE, QUALITY of life, MOSQUITO vectors

Abstract

A successful experience of lymphatic filariasis control in the Republic of Korea is briefly reviewed. Filariasis in the Republic of Korea was exclusively caused by infection with Brugia malayi. Over the past several decades from the 1950s to 2006, many investigators exerted their efforts to detection, treatment, and follow-up of filariasis patients in endemic areas, and to control filariasis. Mass, combined with selective, treatments with diethylcarbamazine to microfilaria positive persons had been made them free from microfilaremia and contributed to significant decrease of the microfilarial density in previously endemic areas. Significant decrease of microfilaria positive cases in an area influenced eventually to the endemicity of filariasis in the relevant locality. Together with remarkable economic growth followed by improvement of environmental and personal hygiene and living standards, the factors stated above have contributed to blocking the transmission cycle of B. malayi and led to disappearance of this mosquito-borne ancient disease in the Republic of Korea. [ABSTRACT FROM AUTHOR]

Published

2009

210. A Locally Acquired Falciparum Malaria via Nosocomial Transmission in Korea.

Author

Jung-Yeon Kim, Jeong-Su Kim, Mi-Hyun Park, Young-A Kang, Jun-Wook Kwon, Shin-Hyeong Cho, Byeong-Chul Lee, Tong-Soo Kim, and Jong-Koo Lee

Subjects

MALARIA, PLASMODIUM falciparum, NOSOCOMIAL infections, HEMORRHAGE, OLDER men, DISEASES in older people

Abstract

A 57-year old man who was admitted to an emergency room of a tertiary hospital with hemoptysis developed malarial fever 19 days later and then died from severe falciparum malaria 2 days later. He had not traveled outside of Korea for over 30 years. Through intensive interviews and epidemiological surveys, we found that a foreign patient with a recent history of travel to Africa was transferred to the same hospital with severe falciparum malaria. We confirmed through molecular genotyping of the MSP-1 gene that Plasmodium falciparum genotypes of the 2 patients were identical. It is suggested that a breach of standard infection control precautions resulted in this P. falciparum transmission between 2 patients in a hospital environment. This is the first report of a nosocomial transmission of falciparum malaria in Korea. [ABSTRACT FROM AUTHOR]

Published

2009

211. A Nationwide Survey on the Prevalence of Intestinal Parasitic Infections in the Republic of Korea, 2004.

Author

Tong-Soo Kim, Shin-Hyeong Cho, Sun Huh, Yoon Kong, Woon-Mok Sohn, Seung-Sik Hwang, Jong-Yil Chai, Soon-Hyung Lee, Yun-Kyu Park, Dae-Kyu Oh, and Jong-Koo Lee

Subjects

DISEASE prevalence, PARASITIC diseases, INTESTINAL diseases, FECES examination, HEALTH surveys

Abstract

National surveys on the prevalence of intestinal parasitic infections have been carried out every 5-7 years since 1971 in the Republic of Korea in order to establish control measures. The present nationwide survey was conducted from June to December 2004. The 10% population sampling data of Population and Housing Census by the Korean government in 2000 was used as the survey population. One sample was selected randomly from each of the 22,858 registered subjects, and a total of 20,541 people were ultimately included in this survey. Fecal examinations were performed by the cellophane thick smear and saturated brine flotation techniques. Pinworm infection was examined by cello-tape anal swab method. This survey also included a questionnaire study for a socioeconomic analysis. The total helminth egg positive rate was 3.7%, and the estimated total positive number among nationwide people was 1,780,000. The rates in urban and rural areas were 3.1% and 6.8%, respectively. As the total egg positive rate in the 6th survey in 1997 was 2.4%, the present survey showed that there was a considerable degree of increase in the prevalence rate of intestinal parasitic infections over the 7-year period following the 6th survey. The largest increases occurred in the egg positive rates of Clonorchis sinensis and heterophyids including Metagonimus yokogawai. [ABSTRACT FROM AUTHOR]

Published

2009

212. Identification and characterization of a serine protease inhibitor of Paragonimus westermani.

Author

Jin-Hee Hwang, Wook-Gyo Lee, Byoung-Kuk Na, Hyeong-Woo Lee, Shin-Hyeong Cho, and Tong-Soo Kim

Subjects

HELMINTHS, SERINE proteinase inhibitors, CELLULAR control mechanisms, GRANULOMA, GENETIC code, BIOCHEMISTRY, RECOMBINANT proteins, BACTERIAL proteins

Abstract

Abstract   Paragonimus westermani is a trematode parasite that causes pulmonary and/or extrapulmonary granulomatous disease in humans. In this study, we identified a full-length gene encoding a novel serine protease inhibitor of P. westermani (PwSERPIN) and characterized the biochemical properties of the recombinant protein. PwSERPIN had an open reading frame of 1,164 bp, which encoded 387 amino acid residues. Sequence analysis of the primary structure of PwSERPIN revealed that it had the essential structural motifs which were well conserved among the serine protease inhibitor (serpin) superfamily and had shown 16.5–29.6% sequence identities with previously reported serpins from other helminthic parasites. No signal peptide or N-glycosylation site was found in the sequence. Genomic DNA structure analysis showed that PwSERPIN comprised six exons separated by five introns. The bacterially expressed recombinant PwSERPIN effectively inhibited the activities of trypsin, thrombin, and chymotrypsin in a dose-dependent manner, but showed lower inhibitory capacity on cathepsin G and elastases. Expression of PwSERPIN was detected throughout various developmental stages of the parasite, from metacercariae to adult worms, and the transcription level gradually increased with the maturation of the parasite. PwSERPIN was identified in the soluble extract of the parasite, but not in the excretory and secretory products (ESP) and in the insoluble extract of the parasite. These results collectively suggest that the PwSERPIN is an intracellular serpin of P. westermani and that might play primary roles in regulating the activities of intracellular serine proteases of the parasite. [ABSTRACT FROM AUTHOR]

Published

2009

213. High Levels of Antibodies to Plasmodium falciparum Liver Stage Antigen-1 in Naturally Infected Individuals in Myanmar.

Author

Hyeong-Woo Lee, Sung-Ung Moon, Yeon-Joo Kim, Shin-Hyeong Cho, Khin Lin, Byoung-Kuk Na, and Tong-Soo Kim

Subjects

IMMUNOGLOBULINS, PLASMODIUM falciparum, PARASITE antigens, IMMUNOGLOBULIN G, PROTEINS, VACCINES

Abstract

Plasmodium falciparum liver stage antigen-1 (PfLSA-1) is one of the few antigens expressed exclusively in liver stage parasites. In this study, we evaluated the antibody responses against recombinant PfLSA-1 in naturally infected individuals in Myanmar. High levels of antibody responses (70.7%) were detected in 82 serum samples from 116 infected individuals, and IgG responses to PfLSA-1 principally composed of responses of IgG1 and IgG3 subclasses. These results show that PfLSA-1 elicits effective antibody responses in individuals infected with P. falciparum, and thus it could be not only an attractive candidate protein for vaccine development, but also a useful antigen for serodiagnosis of the infection. [ABSTRACT FROM AUTHOR]

Published

2008

214. Larval Gnathostoma hispidum detected in the red banded odd-tooth snake, Dinodon rufozonatum rufozonatum, from China.

Author

Shin-Hyeong CHO, Tong-Soo Kim, Yoon Kong, Byoung-Kuk Na, and Woon-Mok Sohn

Subjects

GNATHOSTOMA, SNAKES, LARVAE, MICROSCOPES, SCANNING electron microscopy

Abstract

A total of 205 larval gnathostomes were collected from 18 (22.5%) of 80 red banded odd-tooth snakes, Dinodon rufozonatum rufozonatum, which had been smuggled from China and confiscated at Customs in Busan, Republic of Korea. In order to identify the species, some of the larvae were observed by a light microscope and a scanning electron microscope (SEM). The larvae were 2.18 x 0.29 mm in average size, and had a pair of lips at the anterior end, a muscular esophagus, 2 pairs of cervical sacs, and brownish intestines. The head bulb was characteristically equipped with 4 rows of hooklets; the average number of hooklets in each respective row was 38.6, 40.5, 41.5, and 43.7. In SEM views, the mouth evidenced a pair of lateral lips of equal size in a half-moon shape. Each lip featured a couple of labial papillae and a small amphid located between the 2 papillae. The hooklets on the head bulb had single-pointed, posteriorly-curved tips. The cuticular spines were larger and more densely distributed on the anterior part of the body, and decreased gradually in size and number toward the posterior body. On the basis of these morphological characteristics, the larvae were identified as the third stage larvae of Gnathostoma hispidum. [ABSTRACT FROM AUTHOR]

Published

2007

215. Arthrostoma miyazakiense (Nematoda: Ancylostomatidae) infection in raccoon dogs of Korea and experimental transmission to dogs.

Author

Sung-Shik Shin, Dae-Jung Cha, Kyoung-Oh Cho, Ho-Sung Cho, Jeong-Ok Choi, and Shin-Hyeong Cho

Subjects

NEMATODES, ANCYLOSTOMATIDAE, HOOKWORMS, HOOKWORM disease, RACCOON dog, HELMINTHS, GIARDIA

Abstract

Arthrostoma miyazakiense (Nematoda: Ancylostomatidae) is a hookworm species reported from the small intestines of raccoon dogs (Nyctereutes procyonoides) in Japan. Five Korean raccoon dogs (N. procyonoides koreensis) caught from 2002 to 2005 in Jeollanam-do (Province), a southeastern area of South Korea, contained helminth eggs belonging to 4 genera (roundworm, hookworm, whipworm, and Capillaria spp.) and cysts of Giardia sp. in their feces. Necropsy findings of 1 raccoon dog revealed a large number of adult hookworms in the duodenum. These hookworms were identified as Arthrostoma miyazakiense based on the 10 articulated plates observed in the buccal capsule and the presence of right-sided prevulval papillae. Eggs of A. miyazakiense were 60-65 x 35-40 µm (av. 62.5 x 35 µm, and were morphologically indistinguishable from those of Ancylostoma caninum. The eggs were cultured to infective 2nd stage larvae via charcoal culture, and 100 infective larvae were used to experimentally infect each of 3 mixed-bred puppies. All puppies harbored hookworm eggs in their feces on the 12th day after infection. This is the first report thus far concerning A. miyazakiense infections in raccoon dogs in Korea, and the first such report outside of Japan. [ABSTRACT FROM AUTHOR]

Published

2007

216. MOLECULAR CLONING AND CHARACTERIZATION OF COPPER/ZINC-SUPEROXIDE DISMUTASE OF PARAGONIMUS WESTERMANI.

Author

Ai-Hua Li, Byoung-Kuk Na, Yoon Kong, Shin-Hyeong Cho, Qin Ping Zhao, and Tong-Soo Kim

Subjects

PARAGONIMUS, MOLECULAR cloning, SUPEROXIDE dismutase, PARASITES, HOST-parasite relationships, DNA, ESCHERICHIA coli, AMINO acid sequence

Abstract

Discusses the molecular cloning and characterization of copper/zinc-superoxide dismutase of Paragonimus westermani. Roles of superoxide dismutases in the protection of the parasites against cellular oxygen-mediated killing of the hosts; Isolation of a DNA encoding a copper/zinc-superoxide; Expression of the active enzyme in Escherichia coli; Biochemical properties. Deduced amino acid sequence of the gene.

Published

2005

217. The First Outbreak of Giardiasis with Drinking Water in Korea

Author

Cheon-Hyeon Kim, Hyeng-Il Cheun, Da-Won Ma, Mun-Su Na, Shin-Hyeong Cho, Seung-Ki Youn, Bo-La Goo, and Won-Ja Lee

Subjects

Veterinary medicine, business.industry, water-borne outbreak, Public Health, Environmental and Occupational Health, Outbreak, Water supply, Waterborne diseases, medicine.disease_cause, medicine.disease, DNA extraction, Diarrhea, giardiasis, Infectious Diseases, fluids and secretions, parasitic diseases, medicine, Giardia lamblia, Original Article, medicine.symptom, business, Feces, Building construction

Abstract

Objectives To identify the pathogen of the diarrhea outbreak in a village in Jeollabuk province in Korea in April 2010. Methods DNA extraction was performed from the 120 L of collected water, which was centrifuged at 10,000 x g for 30 min. PCR reactions were conducted in a total of 25 ul, which included PCR premix (GenDEPOT, Barker, TX, USA), 2 ul (∼100 ng) of extracted DNA, and 10 pmol of each primer. Results Nine people out of 25 had a symptom of abdominal pain accompanied by diarrhea after they used stored valley water in a water tank as a provisional water supply source without chlorine sterilization. Among them Giardia lamblia was detected in fecal samples of 7 people using the polymerase chain reaction method. Although G. lamblia was also detected from water provided by the provisional water supply system stored in the water tank and used as drinking water, it was not detected in the water tank itself. This water-borne outbreak is considered to have occurred when the provisional water supply tube was destroyed under a building construction and contaminated by G. lamblia , but its precise cause has not been clarified. Conclusion This outbreak resulting from G. lamblia is very meaningful as the first outbreak of an infection by a water-borne parasite in Korea.

218. Induction of IL-10-producing regulatory B cells following Toxoplasma gondii infection is important to the cyst formation

Author

Sang Eun Lee, Young-Il Jeong, Shin-Hyeong Cho, Sung-Hee Hong, and Mi Yeoun Park

Subjects

0301 basic medicine, IL-10-producing regulatory B cell, biology, Transgene, Regulatory B cells, Naive B cell, Biophysics, Toxoplasma gondii, biology.organism_classification, Biochemistry, Microbiology, 03 medical and health sciences, Interleukin 10, Chronic infection, 030104 developmental biology, Immune system, Downregulation and upregulation, Immunology, parasitic diseases

Abstract

Toxoplasma gondii is a protozoan parasite that infects humans and animals via congenital or postnatal routes. During parasite infection, IL-10-producing Bregs are stimulated as part of the parasite-induced host immune responses that favor infection. In this study, we investigated whether T. gondii infection induces immune regulatory cells including IL-10-producing CD1dhighCD5+ regulatory B cells (Bregs) and whether Breg induction is critical for the development of chronic infection of T. gondii. Furthermore, B cell-deficient (μMT) mice revealed that the IL-10-producing B cells might be associated with the development of chronic T. gondii infection. To better understand the mechanism underlying the accumulation of IL-10-producing B cells upon T. gondii infection, we determined the effect of products released by T. gondii on the induction and differentiation of IL-10-producing B cells during the acute stage of infection using transgenic green fluorescent protein (GFP)-expressing T. gondii strain. We demonstrated that products secreted at the stage of cell lysis by fully replicated tachyzoites induced the differentiation of naive B cells to IL-10-producing Bregs. Our results indicated that the downregulation of the immune response via Bregs during T. gondii infection is related to cyst formation in the host brain and to the establishment of chronic infection.

219. Genotype of Toxoplasma gondii from Blood of Stray Cats in Gyeonggi-do, Korea.

Author

Hye-Youn Kim, Yun-Ah Kim, Ho Sa Lee, Ho Gun Rhie, Shin-Hyeong Cho, Jae-Ran Yu, and Sang-Eun Lee

Subjects

TOXOPLASMA gondii, POLYMERASE chain reaction, RESTRICTION fragment length polymorphisms, GENES, CELL surface antigens, CATS

Abstract

Genotyping of Toxoplasma gondii has been performed in 23 PCR positive blood samples from stray cats in Korea. We used 2 separate PCR-restriction fragment length polymorphism (RFLP) patterns of SAG2 gene, amplifying the 5' and 3' ends of the locus. The results revealed that all samples belonged to the type I clonal lineage. Although T. gondii organisms were not isolated from the samples, the results of the present study represent that stray cats with T. gondii infection should be seriously concerned in our environment. Adequate and continuous control programs of stray cats are needed to reduce the risk of transmission of T. gondii as a zoonotic infection threatening the public health. [ABSTRACT FROM AUTHOR]

Published

2009

220. ClonorESTdb: a comprehensive database for Clonorchis sinensis EST sequences

Author

Yu-Jung Kim, Jung-Won Ju, Won-Ja Lee, Shin-Hyeong Cho, Won Gi Yoo, Myoung-Ro Lee, Sanghyun Lee, and Dae-Won Kim

Subjects

Information Storage and Retrieval, Genomics, Biology, Data Note, computer.software_genre, Polymorphism, Single Nucleotide, General Biochemistry, Genetics and Molecular Biology, Database, Databases, Genetic, medicine, Animals, KEGG, Gene Library, Expressed Sequence Tags, Genetics, Medicine(all), Internet, Life Cycle Stages, Expressed sequence tag, Clonorchis sinensis, Biochemistry, Genetics and Molecular Biology(all), Gene Expression Profiling, Expressed sequence tags (ESTs), Computational Biology, General Medicine, biology.organism_classification, medicine.disease, Clonorchiasis, UniProt, Transcriptome, Functional genomics, computer, InterProScan

Abstract

Clonorchiasis, which is primarily caused by liver fluke (Platyhelminthes), is a fatal infectious disease that is mainly associated with bile duct malignancy and the subsequent development of cholangiocarcinoma. Thus, a genomic approach now represents an important step to further our knowledge of biology and the pathology of these parasites. The results of expressed sequence tags (ESTs) sequencing need to be well organized into databases to provide an integrated set of tools and functional information. Here, the ClonorESTdb database represents a collection of Clonorchis sinensis ESTs that is intended as a resource for parasite functional genomics. A total of 55,736 successful EST sequences, which are cleaned and clustered into non-redundant 13,305 C. sinensis assembled EST sequences (6,497 clusters and 6,808 singletons), were obtained from three in-house prepared cDNA libraries of C. sinensis at different developmental stages. The assembled consensus sequences were annotated using the BLAST algorithm or/and hmm against NCBI NR, UniProt, KEGG and InterProScan. The ClonorESTdb database provides functional annotation, their expression profiles, tandem repeats and putative single nucleotide polymorphisms with utility tools such as local BLAST search and text retrieval. This resource enables the researcher to identify and compare expression signatures under different biological stages and promotes ongoing parasite drug and vaccine development and biological research. Database URL: http://pathod.cdc.go.kr/clonorestdb/

221. Prevalence of Plasmodium vivax VK210 and VK247 subtype in Myanmar

Author

Sun-Sim Lee, Yoon-Joong Kang, Hyung-Hwan Kim, Tong-Soo Kim, Shin-Hyeong Cho, Byoung-Kuk Na, Khin Lin, Do Kyung Kim, Hyeong-Woo Lee, Hyuck Kim, and Youngjoo Sohn

Subjects

lcsh:Arctic medicine. Tropical medicine, Genotype, lcsh:RC955-962, Molecular Sequence Data, Plasmodium vivax, Protozoan Proteins, Antibodies, Protozoan, Enzyme-Linked Immunosorbent Assay, Myanmar, Polymerase Chain Reaction, lcsh:Infectious and parasitic diseases, law.invention, Serology, Seroepidemiologic Studies, law, parasitic diseases, Malaria, Vivax, Prevalence, medicine, Humans, Serologic Tests, lcsh:RC109-216, Fluorescent Antibody Technique, Indirect, Polymerase chain reaction, biology, Research, Genetic Variation, Plasmodium falciparum, Sequence Analysis, DNA, medicine.disease, biology.organism_classification, Virology, Circumsporozoite protein, Infectious Diseases, Parasitology, biology.protein, Antibody, DNA Probes, Malaria

Abstract

Background Plasmodium vivax is divided into two subtypes, a dominant form, VK210 and a variant form, VK247. This division is dependent on the amino acid composition of the circumsporozoite (CS) protein. In this study, the prevalence of the VK247 variant form of P. vivax was investigated in Myanmar. Methods The existence of malaria parasites in blood samples was determined by microscopic examination, polymerase chain reaction (PCR) and DNA hybridization assays. To test for antibodies against P. vivax and Plasmodium falciparum in blood samples, an indirect immunofluorescence antibody test (IFAT) was performed using asexual blood antigens. An enzyme-linked immunosorbent assay with synthetic VK210 and VK247 antigens was carried out to discriminate between the P. vivax subtypes. Results By thick smear examination, 73 (n = 100) patients were single infected with P. vivax, one with P. falciparum and 13 with both species. By thin smear, 53 patients were single infected with P. vivax, eight with only P. falciparum and 16 with both. Most of the collected blood samples were shown to be P. vivax positive (n = 95) by PCR. All cases that were positive for P. falciparum by PCR (n = 43) were also positive for P. vivax. However, 52 cases were single infected with P. vivax. IFAT showed antibody titres from 1:32 to 1:4,096. Additionally, using specific antibodies for VK210 and VK247, ELISA showed that 12 patients had antibodies for only the VK210 subtype, 4 patients had only VK247 subtype antibodies and 21 patients had antibodies for both subtypes. Using a DNA hybridization test, 47 patients were infected with the VK210 type, one patient was infected with VK247 and 23 patients were infected with both subtypes. Conclusions The proportion of the VK247 subtype in Myanmar was 43.1% (n = 25) among 58 positive cases by serodiagnosis and 25.6% (n = 24) among 94 positive cases by genetic diagnosis. In both diagnostic methods, the infection status of malaria patients is highly diverse with respect to malaria species, and multiple clonal infections are prevalent in Myanmar. Therefore, the complexity of the infection should be considered carefully when diagnosing malaria in Myanmar.

222. Genetic polymorphism of merozoite surface protein-1 and merozoite surface protein-2 in Plasmodium falciparum field isolates from Myanmar

Author

Sung-Ung Moon, Woon-Mok Sohn, Shin-Hyeong Cho, Khin Lin, Jung-Mi Kang, Tong-Soo Kim, Jung-Yeon Kim, and Byoung-Kuk Na

Subjects

lcsh:Arctic medicine. Tropical medicine, Genotype, lcsh:RC955-962, Sequence analysis, Plasmodium falciparum, Population, Protozoan Proteins, Antigens, Protozoan, Myanmar, Polymerase Chain Reaction, complex mixtures, lcsh:Infectious and parasitic diseases, parasitic diseases, Humans, lcsh:RC109-216, Malaria, Falciparum, Merozoite surface protein, Allele, education, neoplasms, Alleles, Merozoite Surface Protein 1, Genetics, education.field_of_study, Polymorphism, Genetic, biology, Malaria vaccine, Research, Sequence Analysis, DNA, biology.organism_classification, Virology, Infectious Diseases, Parasitology

Abstract

Background Merozoite surface protein-1 (MSP-1) and MSP-2 of Plasmodium falciparum are potential vaccine candidate antigens for malaria vaccine development. However, extensive genetic polymorphism of the antigens in field isolates of P. falciparum represents a major obstacle for the development of an effective vaccine. In this study, genetic polymorphism of MSP-1 and MSP-2 among P. falciparum field isolates from Myanmar was analysed. Methods A total of 63 P. falciparum infected blood samples, which were collected from patients attending a regional hospital in Mandalay Division, Myanmar, were used in this study. The regions flanking the highly polymorphic characters, block 2 for MSP-1 and block 3 for MSP-2, were genotyped by allele-specific nested-PCR to analyse the population diversity of the parasite. Sequence analysis of the polymorphic regions of MSP-1 and MSP-2 was also conducted to identify allelic diversity in the parasite population. Results Diverse allelic polymorphism of MSP-1 and MSP-2 was identified in P. falciparum isolates from Myanmar and most of the infections were determined to be mixed infections. Sequence analysis of MSP-1 block 2 revealed that 14 different alleles for MSP-1 (5 for K1 type and 9 for MAD20 type) were identified. For MSP-2 block 3, a total of 22 alleles (7 for FC27 type and 15 for 3D7 type) were identified. Conclusion Extensive genetic polymorphism with diverse allele types was identified in MSP-1 and MSP-2 in P. falciparum field isolates from Myanmar. A high level of mixed infections was also observed, as was a high degree of multiplicity of infection.