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251. [Determination of As, Sb, Bi, Cd and Sn in soils and sediments by inductively coupled plasma atomic emission spectrometry after sublimation separation as iodides].

Author

He HL, Hu MY, Gong AH, Wen HL, and Que SJ

Abstract

A method was developed for the determination of As, Sb, Bi, Cd and Sn in degrees C, iodides of As, Sb, Bi, Cd and Sn were formed and sublimated from the sample matrix and then extracted by diluted HCl. The prepared solution was determined by ICP-AES. The sample treatment procedure, such as the ratio of NH4 I to sample, and sublimation and extraction conditions, was studied. The instrument determination parameters, including ICP power, Ar gas flow rate, spectral wavelengths, background subtraction, spectral interferences correction and internal standard, were selected and optimized. The established procedure is rapid and simple, the detection limits for the five elements are in the range of 0.01-0.35 microg x g(-1), and the analytical results for soil and sediment reference materials were in good agreement with the reference values.

Published
2008

252. [Determination of Si, Al and other in biological samples by ICP-AES with fusion with LiBO2 after dry ashing].

Author

Sun DZ, He HL, Wen HL, Ma SF, Gong AH, and Yin SQ

Subjects
Aluminum chemistry, Food Analysis, Limit of Detection, Organosilicon Compounds chemistry, Plants chemistry, Reference Standards, Silicon chemistry, Solvents chemistry, Temperature, Aluminum analysis, Borates chemistry, Lithium chemistry, Silicon analysis, Spectrophotometry, Atomic standards
Abstract

An alkaline sample digestion procedure using fusion with lithium metaborate (LiBO2) after dry ashing was developed. Silicon, aluminium and other, a total of 10 elements in different kinds of biological samples, were measured by ICP-AES. The detection limit of this method was 0.15 microg x mL(-1) for Si and 0.03 microg x mL(-1) for Al. The accuracy and precision of the method were demonstrated by analyzing certified reference materials poplar leaves (GBW07604). The precision was less than 3% and the accuracy was -0.03% for Si and -3% for Al. This method was applied to the certification of a series of ten biological reference materials. The results were satisfied.

Published
2008

253. High throughput and rapid screening of marine protein hydrolysates enriched in peptides with angiotensin-I-converting enzyme inhibitory activity by capillary electrophoresis.

Author

He HL, Chen XL, Wu H, Sun CY, Zhang YZ, and Zhou BC

Subjects
Animals, Bone and Bones chemistry, Cyanobacteria chemistry, Decapoda chemistry, Eukaryota chemistry, Fishes, Meat, Skin chemistry, Angiotensin-Converting Enzyme Inhibitors chemistry, Angiotensin-Converting Enzyme Inhibitors pharmacology, Peptides chemistry, Peptides pharmacology, Protein Hydrolysates chemistry, Protein Hydrolysates pharmacology
Abstract

Twelve kinds of marine protein materials, including fish, shrimp, seashell, algae and seafood wastes were selected for the hydrolysis using four different proteases. The IC(50) values for angiotensin-converting enzyme (ACE) inhibitory activity of 48 hydrolysates were rapidly determined by capillary electrophoresis (CE). The values ranged from 0.17 to 501.7mg/ml, and were affected by both the marine protein resources and the selected proteases. Hydrolysates of the lowest IC(50) values were from shrimp (Acetes chinensis), shark meat, mackerel bone, Polysiphonia urceolata and Spirulina platensis, indicating these five kinds of marine food proteins contained beneficial materials for the production of ACE inhibitory peptides by proteolysis. The hydrolysates obtained using proteases Protamex and SM98011 had lower IC(50) values, showing these two proteases were superior to others. The CE method achieved the same sensitivity as the high performance liquid chromatography (HPLC) method. However, the CE method was faster and, as a result, more economical. Therefore, CE had potential for rapid screening of marine protein hydrolysates enriched in ACE inhibitory peptides.

Published
2007
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255. A novel type of subtilase from the psychrotolerant bacterium Pseudoalteromonas sp. SM9913: catalytic and structural properties of deseasin MCP-01.

Author

Chen XL, Xie BB, Lu JT, He HL, and Zhang Y

Subjects
Binding Sites, Catalytic Domain, Cold Temperature, Molecular Sequence Data, Protein Conformation, Subtilisins chemistry, Endopeptidases chemistry, Endopeptidases metabolism, Pseudoalteromonas enzymology
Abstract

MCP-01, the main protease secreted by the deep-sea cold-adapted bacterium Pseudoalteromonas sp. SM9913, is a cold-adapted serine protease. Gene mcp01 encoding MCP-01 contains an ORF of 2508 bp encoding a protein of 835 amino acid residues with an M(r) of 87 773 Da, which is a multidomain subtilase precursor. Mature MCP-01 purified from the culture of strain SM9913 with an M(r) of 65.84 kDa is a multidomain protein composed of a catalytic domain, a linker, a P_proprotein domain and a polycystic kidney disease (PKD) domain. To the best of the authors' knowledge, no mature subtilase has been reported to date with this domain architecture. Phylogenetic analyses of subtilases showed that MCP-01 and 12 hypothetical proteins retrieved from public databases form a strongly supported group within the subtilase subfamily. These 13 proteins are predicted to share a similar domain architecture and represent a structurally novel group within the S8A subfamily. The substrate specificities of MCP-01 towards synthetic peptides differed from that of a typical S8A protease, subtilisin Carlsberg. Since most of this new subgroup of subtilases, including MCP-01 and the 12 MCP-01-like subtilases, are from deep-sea bacteria, they are termed deseasins. MCP-01 is the type example of a deseasin, since it is the only one that has been purified and characterized. In addition, the structural characteristics and catalytic properties of deseasin MCP-01 show that structurally and kinetically it is adapted to low temperatures.

Published
2007
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257. [Treatment of bilateral cervical facet dislocation by reduction through anterior distraction].

Author

He HL, Ye XJ, Tan JM, Li JS, Jia LS, Chen DY, Ni B, and Yuan W

Subjects
Adult, Female, Follow-Up Studies, Humans, Male, Middle Aged, Treatment Outcome, Cervical Vertebrae, Joint Dislocations surgery, Spinal Fusion methods, Zygapophyseal Joint surgery
Abstract

Objective: To investigate the effect of reduction through anterior distraction in treatment of bilateral cervical facet dislocation., Methods: Twenty-one patients with bilateral cervical facet dislocation underwent leverage reduction through anterior distraction, interbody fusion, and internal fixation. Follow-up lasted 16 months (4 months to 5 years)., Results: All of the 21 patients got reduction of cervical facet dislocation and bony fusion. The neurological deficiency in 4 of the 21 patients improved., Conclusion: Simple and safe, reduction through anterior distraction is effective in treatment of bilateral cervical facet dislocation with reliable fusion.

Published
2007

258. [Quality comparison between two cultivated Chinese yam-Kunming yam and Tiegun yam].

Author

Zhang WM, Shan CY, He HL, Jiang HF, and Zhang J

Subjects
China, Dioscorea growth & development, Fats analysis, Fats isolation & purification, Plant Proteins isolation & purification, Plant Tubers chemistry, Plant Tubers growth & development, Plants, Edible chemistry, Plants, Edible growth & development, Plants, Medicinal growth & development, Polysaccharides isolation & purification, Quality Control, Species Specificity, Dioscorea chemistry, Plant Proteins analysis, Plants, Medicinal chemistry, Polysaccharides analysis
Abstract

Objective: To compare the quality of cultivated Chinese yam (Dioscorea polystachya Turcz.) from Yunnan (Kunming yam) and Henan (Tiegum yam) by determining the content of dry substance in fresh sample and the contents of water extracts, ethanol extracts, starch, protein, crude-fat and polysaccharide in dry sample., Method: The above-mentioned indexes were determined by methods of air desiccation, cold-immersing, hot-immersing, iodine-blue coloration, half Micro-Kjeldahl, Soxhlet extraction and spectrophotometric method respectively., Result: In fresh sample, the content of dry substance of Kunming yam is a little lower than Tiegun yam; in dry sample, all indexes of Kunming yam are higher than or approach to those of Tiegun yam except the content of crude-fat. Especially the content of polysaccharide in Kunming yam is 64% higher than that of Tiegun yam., Conclusion: Kunming yam, with high quality, high yield and good taste, deserves paying close attention as a good variety.

Published
2007

259. Do the lungs contribute to propofol elimination in patients during orthotopic liver transplantation without veno-venous bypass?

Author

Chen YZ, Zhu SM, He HL, Xu JH, Huang SQ, and Chen QL

Subjects
Adult, Anesthetics, Intravenous blood, Female, Humans, Male, Middle Aged, Propofol blood, Pulmonary Artery, Radial Artery, Anesthetics, Intravenous pharmacokinetics, Liver Transplantation, Lung metabolism, Propofol pharmacokinetics
Abstract

Background: The clearance of propofol is very rapid, and its transformation takes place mainly in the liver. Some reports indicated extrahepatic clearance of the drug and that the lungs are the likely place where the process occurs. This study was undertaken to compare the plasma concentrations of propofol both in the pulmonary and radial arteries after constant infusion during the dissection, anhepatic and reperfusion phases of orthotopic liver transplantation (OLT) without veno-venous bypass, attempting to investigate extrahepatic clearance and to determine whether the human lungs take part in the elimination of propofol., Methods: Fifteen patients undergoing OLT without veno-venous bypass were enrolled in the study, and propofol was infused via a forearm vein at a rate of 2 mg x kg-1 x h-1. Blood samples were simultaneously collected from pulmonary and radial arteries at the end of the first hepatic portal dissection (T0), at the clamping of the portal vein (T1), 30, and 60 minutes after the beginning of the anhepatic phase (T2, T3), and 30, 60, and 120 minutes after the unclamping of the new liver (T4, T5, T6). Plasma propofol concentrations were measured using a reversed-phase, high-performance liquid chromatographic method with fluorescence detection., Results: The concentrations of plasma propofol in the pulmonary and radial arteries at T2 and T3 rose significantly compared with T0 and T1 (P<0.01) respectively. After reperfusion, the drug concentrations at T4, T5 and T6 decreased significantly compared with T2, T3 (P<0.01) respectively. There were no significant differences in plasma propofol concentrations between the pulmonary and radial arteries at any time points., Conclusions: Propofol is eliminated mainly by the liver, and also by extrahepatic organs. The lungs seem to be not a major site contributing to the extrahepatic metabolism of propofol in humans.

Published
2006

260. [Detection of fusion genes resulting from chromosome abnormalities in childhood acute lymphoblastic leukemia].

Author

He J, Chen ZX, Xue YQ, Li JQ, He HL, Huang YP, He YX, Chai YH, and Zhu LL

Subjects
Adolescent, Child, Child, Preschool, Core Binding Factor Alpha 2 Subunit genetics, Core Binding Factor Alpha 2 Subunit metabolism, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Flow Cytometry, Homeodomain Proteins genetics, Homeodomain Proteins metabolism, Humans, Immunophenotyping, Infant, Karyotyping, Myeloid-Lymphoid Leukemia Protein genetics, Myeloid-Lymphoid Leukemia Protein metabolism, Oncogene Proteins, Fusion metabolism, Precursor Cell Lymphoblastic Leukemia-Lymphoma metabolism, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins metabolism, RNA-Binding Protein FUS genetics, RNA-Binding Protein FUS metabolism, Reverse Transcriptase Polymerase Chain Reaction, Transcription Factors genetics, Transcription Factors metabolism, Chromosome Aberrations, Oncogene Proteins, Fusion genetics, Precursor Cell Lymphoblastic Leukemia-Lymphoma genetics
Abstract

Objective: To detect the expression of the fusion genes resulting from chromosome abnormalities in childhood acute lymphoblastic leukemia(ALL) and its conformity to WHO classification., Methods: Sixty-two children with ALL were investigated. The expression of fusion genes was determined by multiplex reverse transcription-polymerase chain reaction (RT-PCR), karyotyping (R band) and immunophenotyping (by flow cytometry) were also performed., Results: Of the 62 patients, 23(37.1%) were found to carry 13 different fusion genes. The patients with immunophenotype of Pre-B-ALL were found to carry: TEL/AML1(3 cases); E2A/PBX1, E2A/HLF, TLS/ERG, MLL/AF4, MLL/AF9, MLL/AF10, MLL/AFX-MLL/AF6-MLL/ELL, MLL/AF6-MLL/ELL, dupMLL (one case for each); and HOX11 (6 cases). The patients with immunophenotype of Pre-T-ALL were found to carry: TAL1D (4 cases, one is also found to have HOX11 expression); and HOX11 (2 cases). The multiplex RT-PCR in combination with chromosome analysis revealed genetic abnormalities in 69.4%(43/62) of childhood ALL., Conclusion: Multiplex RT-PCR combined with chromosome analysis and immunophenotyping can provide reliable and helpful information for the diagnosis, therapy evaluation and prognosis prediction in childhood ALL, which may also serve as a basis on which to implement the criteria of WHO classification.

Published
2005

261. Dose requirements of continuous infusion of rocuronium and atracurium throughout orthotopic liver transplantation in humans.

Author

Weng XC, Zhou L, Fu YY, Zhu SM, He HL, and Wu J

Subjects
Adult, Aged, Androstanols pharmacokinetics, Atracurium pharmacokinetics, Humans, Infusions, Intravenous, Intraoperative Period, Liver metabolism, Male, Middle Aged, Neuromuscular Nondepolarizing Agents pharmacokinetics, Rocuronium, Androstanols administration & dosage, Atracurium administration & dosage, Liver Transplantation, Neuromuscular Nondepolarizing Agents administration & dosage
Abstract

Objective: To compare the dose requirements of continuous infusion of rocuronium and atracurium throughout orthotopic liver transplantation (OLT) in humans., Methods: Twenty male patients undergoing liver transplantation were randomly assigned to two comparable groups of 10 patients each to receive a continuous infusion of rocuronium or atracurium under intravenous balanced anesthesia. The response of adductor pollicis to train-of-four (TOF) stimulation of unlar nerve was monitored. The infusion rates of rocuronium and atracurium were adjusted to maintain T1/Tc ratio of 2%~10%. The total dose of each drug given during each of the three phases of OLT was recorded., Results: Rocuronium requirement, which were (0.468+/-0.167) mg/(kg.h) during the paleohepatic phase, decreased significantly during the anhepatic phase to (0.303+/-0.134) mg/(kg.h) and returned to the initial values at the neohepatic period ((0.429+/-0.130) mg/(kg.h)); whereas atracuruim requirements remained unchanged during orthotopic liver transplantation., Conclusions: This study showed that the exclusion of the liver from the circulation results in the significantly reduced requirement of rocuronium while the requirement of atracurium was not changed, which suggests that the liver is of major importance in the clearance of rocuronium. A continuous infusion of atracurium with constant rate can provide stable neuromuscular blockade during the three stages of OLT.

Published
2005
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262. Genome-wide analyses of two families of snoRNA genes from Drosophila melanogaster, demonstrating the extensive utilization of introns for coding of snoRNAs.

Author

Huang ZP, Zhou H, He HL, Chen CL, Liang D, and Qu LH

Subjects
Animals, Base Sequence, Chromosome Mapping, DNA, Complementary genetics, Gene Library, Molecular Sequence Data, Multigene Family, Sequence Homology, Nucleic Acid, Drosophila melanogaster genetics, Genome, Introns genetics, RNA, Small Nucleolar genetics
Abstract

Small nucleolar RNAs (snoRNAs) are an abundant group of noncoding RNAs mainly involved in the post-transcriptional modifications of rRNAs in eukaryotes. In this study, a large-scale genome-wide analysis of the two major families of snoRNA genes in the fruit fly Drosophila melanogaster has been performed using experimental and computational RNomics methods. Two hundred and twelve gene variants, encoding 56 box H/ACA and 63 box C/D snoRNAs, were identified, of which 57 novel snoRNAs have been reported for the first time. These snoRNAs were predicted to guide a total of 147 methylations and pseudouridylations on rRNAs and snRNAs, showing a more comprehensive pattern of rRNA modification in the fruit fly. With the exception of nine, all the snoRNAs identified to date in D. melanogaster are intron encoded. Remarkably, the genomic organization of the snoRNAs is characteristic of 8 dUhg genes and 17 intronic gene clusters, demonstrating that distinct organizations dominate the expression of the two families of snoRNAs in the fruit fly. Of the 267 introns in the host genes, more than half have been identified as host introns for coding of snoRNAs. In contrast to mammals, the variation in size of the host introns is mainly due to differences in the number of snoRNAs they contain. These results demonstrate the extensive utilization of introns for coding of snoRNAs in the host genes and shed light on further research of other noncoding RNA genes in the large introns of the Drosophila genome.

Published
2005
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263. [Study on clinical and biological characteristics of childhood acute leukemia with MLL gene rearrangements].

Author

He J, Chen ZX, Xue YQ, Pan JL, He HL, Li JQ, Wu YF, Huang YP, and Zhu LL

Subjects
Adolescent, Child, Child, Preschool, Female, Humans, In Situ Hybridization, Fluorescence, Infant, Male, Gene Rearrangement, Leukemia genetics, Myeloid-Lymphoid Leukemia Protein genetics
Abstract

Objective: To study the clinical and laboratory features of childhood acute leukemia (AL) with MLL gene rearrangements., Methods: Sixteen of 298 cases of childhood AL with MLL rearrangements were studied by using MLL dual-color FISH, multiplex RT-PCR with 13 pairs of primers in combination with R banding karyotype analysis and cell immunophenotyping by flow cytometry., Results: Sixteen cases of childhood AL with MLL rearrangements accounted for 5.4% of 298 AL patients, and 56.3% of infant ALs. Among 106 cases analyzed by multiplex RT-PCR, MLL gene rearrangements were found in 11 cases, including MLL/AF4 fusion gene in 2, MLL/AF6 fusion gene in 1, MLL/AF6 and MLL/ELL combined with MLL/ AFX or HOX11 in one case each, MLL/AF9 in 2, MLL/AF10 in 1, MLL/ELL in 2. MLL partial tandem duplication in 1 and activated HOX11 in 1. In 27 cases assayed by FISH, 9 cases (36.0%) were demonstrated MLL gene rearrangements. In 16 patients with MLL gene rearrangements, 14 (87.5%) exhibited clonal chromosome abnormalities involved chromosome 11 in 11 cases: being t(4;11) in 2, t(6;11), t(8;11), t(7;8;11), t(9;11) in each trisomy 11 in 2 and 11q--in 3 cases. Among these 16 patients, 11 were B-ALL, and 5 AML-M5, 3 of the latter were CD7+ and CD2+. Of these 16 patients, 8 received chemotherapy and 7 of them achieved complete remission, while the other 8 patients gave up treatment., Conclusion: Multiplex RT-PCR combined with FISH provided a more accurate and sensitive method for detection of MLL gene rearrangements. Finding out MLL gene rearrangement is of most importance in guiding therapy and predicting prognosis in childhood AL.

Published
2005

264. Plasma propofol concentrations during orthotopic liver transplantation.

Author

Wu J, Zhu SM, He HL, Weng XC, Huang SQ, and Chen YZ

Subjects
Adult, Anesthetics, Intravenous administration & dosage, Blood Pressure drug effects, Central Venous Pressure drug effects, Drug Delivery Systems, Female, Heart Rate drug effects, Humans, Infusions, Intravenous, Male, Middle Aged, Monitoring, Intraoperative, Propofol administration & dosage, Anesthetics, Intravenous blood, Liver Transplantation, Propofol blood
Abstract

Objective: The aim of this study was to investigate the changes in plasma concentrations of propofol in three phases (the paleohepatic, anhepatic, and neohepatic phases) during orthotopic liver transplantation (OLT) using target-controlled infusion (TCI)., Methods: Ten patients undergoing OLT without venovenous bypass were studied (age 29-53 years, weight 56-79 kg). After intubation, a non-hypnotic target concentration of propofol 0.5 microg ml(-1) using a Diprifusor pump (Zeneca Pharmaceuticals, Macclesfield, UK) was administered as a supplement anesthesia throughout the procedure. Plasma samples were obtained in each phase for propofol assay, respectively. Performance parameters for the Diprifusor system in each phase, the percentage median performance error (MDPE), the percentage median absolute performance error (MDAPE), and the percentage median absolute constancy error (MDACE) were evaluated., Results: In all patients, measured plasma propofol concentrations were several times higher than Diprifusor values in each phase during the procedure. In nine patients, propofol concentrations in the anhepatic phase were higher than those in the paleohepatic or neohepatic phase (P < 0.05). There were no significant differences between the paleohepatic and neohepatic phases. Interindividual variation of the plasma propofol concentrations was significant (P < 0.05). Percentage median performance error of Diprifusor in each phase, as well as MDAPE, was large (>300%) and was significantly higher in the anhepatic phase (P < 0.01), whereas MDACE was relatively small and there was no significant difference between phases., Conclusions: Models used by Diprifusor are not suitable for liver transplantation patients. A further study should be performed in order to determine all pharmacokinetic parameters of propofol in these patients.

Published
2005
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265. [Therapeutic effectiveness of CCLG-97 protocol on standard-risk childhood acute lymphoblastic leukemia].

Author

Xiao PF, Chai YH, Li JQ, He HL, Wang Y, Li ZP, He YX, and Ji ZH

Subjects
Adolescent, Child, Child, Preschool, China, Disease-Free Survival, Female, Follow-Up Studies, Humans, Infant, Male, Precursor Cell Lymphoblastic Leukemia-Lymphoma mortality, Remission Induction methods, Risk Factors, Secondary Prevention, Survival Rate, Time Factors, Treatment Outcome, Antineoplastic Combined Chemotherapy Protocols therapeutic use, Precursor Cell Lymphoblastic Leukemia-Lymphoma drug therapy, Precursor Cell Lymphoblastic Leukemia-Lymphoma prevention & control
Abstract

Objective: With the improvement of the diagnosis and treatment, the complete remission (CR) rate and the survival rate of childhood acute lymphoblastic leukemia have been increased in the recent 10 years. The objective of this study was to analyze the outcomes of 119 standard-risk childhood acute lymphoblastic leukemia (SR-ALL) patients, and explore how to improve the survival rate in ALL., Methods: A total of 119 patients aged 14 months to 15 years were diagnosed as SR-ALL according to the Suggestion of Diagnosis And Treatment for Childhood Acute Leukemia-1993. Among them, seventy-nine were boys and 40 were girls. All of the patients were treated with the CCLG-97 protocol and were followed up for a period of 20 approximately 78 months., Results: The complete remission rate reached 97.4% in four-week induction. Twenty-one patients were out of follow-up, comprising 63%, 14%, 10%, 8% and 5% of all subjects in 1998, 1999, 2000, 2001 and 2002, respectively. The overall survival rates were 93.3%, 90.2%, 88.0%, 85.0%, 85.0% and 85.0% in 1 year, 2 years, 3 years, 4 years and 5 years, respectively. Relapses occurred in 13 patients (13.8%). Among 9 isolated hematologic relapses, 5 patients (56%) were given irregular therapy, 2 did not reach CR within 4 weeks and relapsed 2 years later, 2 accepted regular therapy, 1 was of hypodiploidy and 1 T-ALL. Isolated central nervous system (CNS) relapse occurred in 4 patients (4.3%). Fifteen patients (12.6%) died, 5 of whom (4.2%) died of complications., Conclusion: Reinforcing administration and regular therapy are important to improve the long-term survival rate in childhood ALL. The clinical classification should be adjusted with the improvement of diagnostic methods. CCLG-97 protocol decreased the rate of the relapses in SR-ALL and didn't increase the rate of therapy-related death. High-dose methotrexate should be used in therapy and its dosage, usage and individualized therapeutic regimen should be further studied.

Published
2005

266. Stabilization of cold-adapted protease MCP-01 promoted by trehalose: prevention of the autolysis.

Author

Pan J, Chen XL, Shun CY, He HL, and Zhang YZ

Subjects
Electrophoresis, Capillary, Endopeptidases chemistry, Enzyme Stability, Temperature, Endopeptidases metabolism, Trehalose pharmacology
Abstract

Protease MCP-01 is similar to other cold-adapted enzymes in that it is a cold-adapted serine protease having high specific activity and low thermostability at low and moderate temperature. Its thermolability and self-autolysis has resulted in difficulties in its purification, preservation and research on its structure and function. The disaccharide trehalose is known to effectively stabilize proteins. Its prevention effect on the autolysis of cold-adapted protease MCP-01 was monitored by capillary electrophoresis. In the absence of trehalose, protease MCP-01 autolyzed rapidly at 35 degrees C. However, when trehalose was added, autolysis was remarkably prevented and the loss of activity reduced. MCP-01 may be a useful model for basic research on the interaction of protein and trehalose.

Published
2005
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267. [The expression of collagen IX in the apical disc of idiopathic scoliosis].

Author

He HL, Wu ZH, Zhang JG, Wang YP, Zhou Y, Xu YQ, Yuan JG, and Qiu GX

Subjects
Adolescent, Adult, Collagen Type IX genetics, Humans, Immunohistochemistry, In Situ Hybridization, RNA, Messenger genetics, Scoliosis genetics, Collagen Type IX metabolism, Intervertebral Disc metabolism, Scoliosis metabolism
Abstract

Objective: To study the distribution of collagen IX gene in the disc and to determine its role in the pathogeny of idiopathic scoliosis (IS)., Methods: The data included apical disc and intermediate disc from 14 cases of adolescent IS, 26 discs from 13 cases of scoliosis of confirmed pathogeny (CPS), which included 10 cases of congenital scoliosis and neurofibromatosis scoliosis. Six discs were obtained from 3 cases of normal young man served as controls. The distribution of collagen IX was studied in the apical disc of IS by immunohistochemistry and in situ hybridization (ISH) with RNA probe. The figure of collagen IX hybridization in the endplate cartilage was input to the figure analysis system. The mRNA content of collagen IX was compared between each group by SPSS software., Results: Collagen IX was mainly distributed in the inner fibrous annulus, nucleus and endplate cartilage. Collagen IX was secreted by the little round chondrocyte-like cells, which was not expressed in the hypertrophic cells. There was significant difference of collagen IX mRNA content between the concave side of apical disc in the IS and the normal disc(P < 0.05), and also between intermediate vertebrae of CS group and normal., Conclusions: There is no obvious abnormal distribution of collagen IX in the disc of idiopathic scoliosis. Collagen IX may be related to the pathogensis of IS. More investigation such as quantity analysis and protein function determination is needed to confirm its role in the pathogenicity of IS.

Published
2005

268. [Primary study on collagen X gene expression in the apical disc of idiopathic scoliosis].

Author

He HL, Wu ZH, Zhang JG, Wang YP, Zhou Y, Xu YQ, Yuan JG, and Qiu GX

Subjects
Adolescent, Adult, Child, Chondrocytes metabolism, Collagen Type X biosynthesis, Female, Genes genetics, Humans, Male, RNA, Messenger biosynthesis, RNA, Messenger genetics, Scoliosis metabolism, Collagen Type X genetics, Intervertebral Disc metabolism, Scoliosis genetics
Abstract

Objective: To study the distribution of collagen X in the intervertebral disc and determine its role in the pathogeny of idiopathic scoliosis (IS)., Methods: The data included apical disc and intermediate disc from 14 cases of AIS, 26 discs from 13 cases of scoliosis of confirmed pathogeny which included 10 cases of congenital scoliosis and neurofibromatosis scoliosis (CS group). Six discs were obtained from 3 cases of sudden death of normal young man served as controls. The distribution of collagen X in the apical disc of IS was examined by immunohistochemistry and in situ hybridization (ISH) with RNA probe. The figure of collagen X hybridization in the endplate cartilage was input to the figure analysis system. The mRNA content of collagen X was compared between every 2 groups by SPSS software., Results: Collagen X was mainly distributed around the hypertrophic chondrocyte in the endplate cartilage. Its mRNA was expressed in the hypertrophic chondrocyte. Positive signal was found in the nuclei of several scoliosis patients, which was not related to the pathogeny. The collagen X mRNA contents of the apical disc and intermediated disc of the IS group and of the CS group were significantly higher than those of the normal group (P < 0.05). There was no difference between the IS and CS groups., Conclusions: Collagen X is mainly distributed around the hypertrophic chondrocyte in the endplate cartilage. Its can also be secreted by the chondrocyte-like cells in the nucleus under special condition. Higher expression of collagn X gene in scoliosis patients may be the effects of long term abnormal stress which causes calcification of endplate cartilage. Collagen X expressed in the nucleus may be the result of secretion of chondrocyte-like cells in the disc under abnormal mechanical condition.

Published
2004

269. [A combined assay of multiplex RT-PCR and karyotypic analysis in childhood acute lymphoblastic leukemia].

Author

He J, Xue YQ, Li JQ, He HL, He YX, Huang YP, Chai YH, and Zhu LL

Subjects
Adolescent, Child, Child, Preschool, Chromosome Aberrations, Female, Humans, Infant, Karyotyping, Male, Precursor Cell Lymphoblastic Leukemia-Lymphoma classification, Reproducibility of Results, Sensitivity and Specificity, Oncogene Proteins, Fusion genetics, Precursor Cell Lymphoblastic Leukemia-Lymphoma diagnosis, Precursor Cell Lymphoblastic Leukemia-Lymphoma genetics, Reverse Transcriptase Polymerase Chain Reaction methods
Abstract

Objective: To study the value of combination assay of multiplex RT-PCR and karyotypic analysis in the diagnosis and classification of childhood acute lymphoblastic leukemia (ALL)., Methods: Fifty cases of childhood ALL patients were studied by multiplex RT-PCR in combination with R or G banding karyotype analysis., Results: Of the 50 childhood ALL patients, 18 (36.0%) carried 11 types of fusion genes including E2A/PBX1, TEL/AML1, TLS/ERG, MLL/AF4, MLL/AF9, MLL/AF10, MLL/AFX, MLL/AF6, MLL/ELL, TAL1D, and HOX11, revealed by multiplex RT-PCR, and in 48 cases, 24 (57.1%) had chromosome abnormalities. Among the latter, numeral chromosome abnormalities and chromosome deletions accounted for 75.0% (18/24), while translocations 25.0% (6/24). The multiplex RT-PCR in combination with chromosome analysis could detect genetic abnormalities in 70% (35/50) of childhood ALL., Conclusions: Multiplex RT-PCR combined with chromosome analysis can enhance the detection rate of genetic abnormalities in childhood ALL. It provides reliable evidence for the diagnosis, classification and prognosis.

Published
2004

270. [Clinical and immunological studies on neonatal infectious pneumonia].

Author

Chen CH, Ye CN, Li MJ, Mao XL, Qiu LF, Lai DM, Yang Q, He HL, and Chen LN

Subjects
Antibodies, Bacterial blood, Antibodies, Viral blood, Bacterial Infections complications, C-Reactive Protein analysis, Enzyme-Linked Immunosorbent Assay, Female, Humans, Infant, Newborn, Male, Pneumonia etiology, T-Lymphocyte Subsets immunology, T-Lymphocyte Subsets metabolism, Virus Diseases complications, Immunoglobulin M blood, Pneumonia diagnosis, Pneumonia immunology
Abstract

Objective: To explore etiology, clinical manifestation and immunological changes of infectious pneumonia of neonates in Chengdu area., Methods: Serum specimens were collected from 111 infants with infectious pneumonia. Eight viral and mycoplasmal specific serum IgM antibodies were detected by enzyme linked immunosorbent assay (ELISA); C reactive protein (CRP), total IgG and its subclasses, IgA and IgM were determined by rate scattered nephelometry; T lymphocyte subpopulations were detected by biotin-streptavidin-peroxidase method, and clinical and other laboratory data were analyzed., Results: (1) Etiological agents: specific serum IgM antibodies were positive in 40 of 111 cases (36.0%) with pneumonias. All the 30 control infants were negative for the specific serum IgM antibodies. Among 111 infants with infectious pneumonia, 20.7% had single viral or mycoplasmal infection, 40.5% had bacterial infection, 15.3% had viral and mycoplasmal infection with bacterial infection; 23.4% had infection with unknown agents. (2) The most common clinical manifestations were tachypnea and cyanosis. The next were cough, milk choking, rales, retractions of the supraclavicular, intercostal and subcostal areas. Roentgenographic examination commonly revealed vague opacities, increased density and patchy infiltration. (3) Immune status: (1) CD(3), CD(4) cell counts of infants with pneumonias were lower than those of the controls while their serum IgA, IgM concentrations were higher than those of the control. (2) The CD(3) and CD(4) cell counts of the group with bacterial infection were lower than those of the control group. (3) The serum IgA concentration of the group with viral and mycoplasmal infection was higher than those of the control group and the group with unknown infection. (4) The serum IgM concentration of the group with bacterial infection was higher than those of the control group. (5) There were no significant differences in CD(8) cell counts, CD(4)/CD(8), concentration of serum IgG and IgG(1 - 4) between pneumonia group and the control group, and among various infectious groups and the control., Conclusion: Pathogens of neonatal infectious pneumonia in Chengdu area included single viral or mycoplasmic infection or bacterial infection, viral and mycoplasmal infection with bacterial infection, and unknown infection. Immunological changes of newborn infants suffered from infectious pneumonia included declined CD(3) and CD(4) cell counts, particularly in bacterial infection.

Published
2003

271. [Clinical and laboratory studies on childhood acute leukemia with 11q23 abnormalities].

Author

He YX, Xue YQ, He J, Zhang XL, Ji ZH, Huang YP, Zhu XM, He HL, Chai YH, and Zhu LL

Subjects
Acute Disease, Adolescent, Child, Child, Preschool, Cytogenetic Analysis, Female, Humans, Immunophenotyping, Infant, Leukemia drug therapy, Leukemia immunology, Male, Prognosis, Retrospective Studies, Chromosome Aberrations, Chromosomes, Human, Pair 11 genetics, Leukemia genetics
Abstract

Objective: To investigate the interrelations among morphology, immunology, cytogenetics and clinical outcome in childhood acute leukemia with 11q23 abnormalities., Methods: Eighteen patients with 11q23 abnormalities, from 320 childhood acute leukemia patients, were retrospectively analysed for cell morphology, flow cytometry, immunophenotyping, R-banding karyotype as well as clinical features and prognosis. Twenty cases of childhood AL with normal karyotype during the same period were used as control., Results: The incidence of 11q23 abnormalities in our childhood acute leukemia patients was 5.63% including 14 acute lymphoblastic leukemia (ALL) and 4 acute myeloid leukemia (AML). Of 16 cases immunophenotypically tested, 13 expressed lymphoid antigens and 3 CD(34) and other myeloid antigens. Karyotype analysis disclosed the following abnormalities: t(4; 11)(q21; q23) in 6 cases, t(10; 11)(p13; q23) in 3, t(11; 19)(q23; p13) in one and del(11)(q23) in 6. The complete remission rate for these patients with 11q23 abnormalities was comparable to that of the control (72.2% vs 80.0%, P > 0.05), while the mortality rate in the former was significantly higher than that in the latter (61.1% vs 25.0%, P < 0.05)., Conclusions: 11q23 abnormalities were mainly seen in childhood ALL and acute monocytic leukemia with unique prognostic features.

Published
2003

272. [The research of estrogen receptor modulator and correlative Chinese herbs].

Author

He HL, Jin H, Wang JF, and Niu JZ

Subjects
Aging drug effects, Animals, Antineoplastic Agents, Phytogenic isolation & purification, Antineoplastic Agents, Phytogenic pharmacology, Coumarins isolation & purification, Coumarins pharmacology, Drugs, Chinese Herbal isolation & purification, Genistein isolation & purification, Genistein pharmacology, Humans, Lignans isolation & purification, Lignans pharmacology, Selective Estrogen Receptor Modulators isolation & purification, Drugs, Chinese Herbal pharmacology, Plants, Medicinal chemistry, Selective Estrogen Receptor Modulators pharmacology
Abstract

Objective: To review the study of estrogen receptor modulator and correlative Chinese herbs., Method: Based on to the documents in the world, the estrogen receptor modulator and correlative Chinese herbs summarized., Result and Conclusion: Estrogen receptor modulator is biological compounds in botany. It can exert faint estrogen-like effects by low affinity with estrogen receptor. Some of the Chinese herbs have the estrogen-like activity, but further and more systemic research work are to be done.

Published
2002

273. [Variations in chromosomal number of regenerated melon plants from somatic embryos].

Author

He HL, Cai R, and Pan JS

Abstract

Chromosomal number of different of somatic embryos regenerated plants were investigated in melon variety "xiaomaigua" and "Qingpilurou". Certain variations of chromosomal number were found among the regenerated plants compared with normal sample,and range of variation covered from 2n = 23-24 to 2n = 13-48 with the increase of generation,the rate from 3.3% to 30%. The results indicated that degree of variation in chromosomal number of somatic embryos regenerated melon plants increased with the time of culture, and those cultured in one to two months had the least variation. It was also found that degree of chromosomal number variations varied with melon varieties.

Published
2002

274. [Changes of motor evoked potentials after spinal cord injuries in rats].

Author

Yu KW, Ye XJ, Li JS, Rong WF, Ja LS, and He HL

Subjects
Animals, Electric Stimulation, Male, Rats, Rats, Sprague-Dawley, Spinal Cord Injuries pathology, Evoked Potentials, Motor physiology, Spinal Cord Injuries physiopathology
Abstract

Aim: Study on the relationship between the degraded spinal cord injuries and the changes of the motor evoked potentials (MEP) to prove the diagnosis and prognosis value of MEP., Methods: After injury at T8-T9 cord using modified Allen's weight-drop method, 27 male SD rats were divided randomly into control group (n = 5), group A (50 gcf, n = 8), group B (70 gcf, n = 8) and group C (100 gcf, n = 6). MEPs elicited by monopolar transcortical stimulation were recorded continuously before injury, just after injury, 15 minutes, 1 hour, 3 hours and 6 hours after injury. The rate of the size of the bleeding or necrosis area to the total cord was also calculated., Results: MEP had no significant change in the control group. The amplitude of MEP's early components in group A or group B decreased or even obliterated after SCI, and then partially recovered, while the late components were lost without any recovery signals. All animals in group C showed no MEP waves excepting 2 rats had recovery signals. The size of the cord injuries area increased according to the dropping force and was correlated significantly with the amplitude of the largest peaks of scMEP 1 hour after SCI (r = -0.821)., Conclusion: The scMEP changes after SCI are correlated with the injury forces and the pathological changes in the cord, which indicates that scMEP can be used as an objective index for the cord functional monitoring.

Published
2002

275. Modeling gene expression with differential equations.

Author

Chen T, He HL, and Church GM

Subjects
Computational Biology methods, Kinetics, Protein Biosynthesis, Transcription, Genetic, Gene Expression, Models, Genetic
Abstract

We propose a differential equation model for gene expression and provide two methods to construct the model from a set of temporal data. We model both transcription and translation by kinetic equations with feedback loops from translation products to transcription. Degradation of proteins and mRNAs is also incorporated. We study two methods to construct the model from experimental data: Minimum Weight Solutions to Linear Equations (MWSLE), which determines the regulation by solving under-determined linear equations, and Fourier Transform for Stable Systems (FTSS), which refines the model with cell cycle constraints. The results suggest that a minor set of temporal data may be sufficient to construct the model at the genome level. We also give a comprehensive discussion of other extended models: the RNA Model, the Protein Model, and the Time Delay Model.

Published
1999

276. Identification of a novel gene expressed in activated natural killer cells and T cells.

Author

Dahl CA, Schall RP, He HL, and Cairns JS

Subjects
Amino Acid Sequence, Base Sequence, DNA isolation & purification, Humans, Killer Cells, Natural immunology, Molecular Sequence Data, T-Lymphocytes immunology, Transcription, Genetic, Gene Expression, Killer Cells, Natural metabolism, Lymphocyte Activation, T-Lymphocytes metabolism
Abstract

We have isolated a cDNA clone from a human activated NK cell-derived cDNA library that identifies a transcript (NK4) that is selectively expressed in lymphocytes. The expression of this transcript is increased after activation of T cells by mitogens or activation of NK cells by IL-2 (lymphokine-activated killer cells). The transcript levels demonstrated by Northern blot analysis increase by 12 h after activation, remain high for at least 48 h, and require protein synthesis for expression. Southern blot analysis of B lymphoblastoid lines derived from 18 unrelated individuals reveal variable banding patterns suggestive of polymorphism within the NK4 gene. No homology was found between the sequence of the coding region of this transcript and any sequences in the GenBank data base. Sequence homology to the U1 small nuclear RNA was found within the 3' untranslated region immediately upstream of the site of polyadenylation, suggesting a possible role for U1 in the polyadenylation process. Sequence analysis indicates the transcript would encode a protein having a mass of 27 kDa. The presence of a signal sequence and lack of a transmembrane region suggests that the protein is secreted. In addition, the protein contains an RGD sequence that may be involved in cellular adhesion. This transcript appears to encode a novel product common to the activation pathways of both NK cells and T cells.

Published
1992

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