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31.
F(ab')2 fragments, herein designated as F(ab')2μ fragments, were prepared from a mouse IgM monoclonal antibody specific to
sialyl Lewis A antigen. The fragments were applied to flow cytometry to analyze the antigen on human cancer cells. The binding
of the fragments to the antigen-positive cells was stronger than that of the original IgM. The non-specific binding of the
IgM antibody to the antigen-negative cells was much decreased by using the F(ab')2μ fragments. These results indicate that
the F(ab')2μ fragments are more suitable than the original IgM monoclonal antibody in flow cytometric analysis.
This revised version was published online in July 2006 with corrections to the Cover Date. 相似文献
32.
Tomio Tada Yoichiro Kondo Ko Okumura Motohito Sano Muneo Yokogawa 《Experimental parasitology》1975,38(3):291-302
Macaca monkeys experimentally infected with Schistosoma japonicum developed a chronic progressive kidney lesion characterized by an increase of mesangial matrix, local glomerular hypercellularity, and local thickening of glomerular basement membrane. Immunofluorescence studies revealed the localization of IgG, IgM, IgA, and IgE immunoglobulins mostly in the mesangial area of the glomeruli accompanied by the deposition of Schistosoma antigens. By electron microscopy, in addition to the local thickening of the glomerular basement membrane, dense homogeneous deposits and those with moth-eaten appearance were detected in the mesangial matrix. These findings suggest that worms in the bloodstream continuously release antigenic materials that stimulate host's antibody response belonging to various immunoglobulin classes including IgE. The produced antibodies and antigens would form immune complexes that deposited in the glomeruli. The increased vascular permeability caused by antigen-IgE antibody interaction may play an important role in the deposition of immune complexes and in the rapid development of kidney injury. 相似文献
33.
A Cahour P Debeire L Hartmann J Montreuil H van Halbeek J F Vliegenthart 《FEBS letters》1984,170(2):343-349
The carbohydrate chains of the pathological human immunoglobulins M from two patients with Waldenström's macroglobulinemia were released by hydrazinolysis. The N-acetyllactosamine-type glycans were obtained by affinity chromatography on concanavalin A and fractionated by high-voltage paper electrophoresis. The primary structure of the major compounds was elucidated on the basis of carbohydrate analysis, methylation analysis, including mass-spectrometry, and 500 MHz 1H-NMR spectroscopy. For both patients, this appeared to be a monosialyl monofucosyl biantennary structure; the compounds differed by the presence of an intersecting N-acetylglucosamine residue. 相似文献
34.
David A. Zarling Donna J. Arndt-Jovin Michel Robert-Nicoud Lawrence P. McIntosh Ralf Thomae Thomas M. Jovin 《Journal of molecular biology》1984,176(3):369-415
The relative immunogenicities of the poly[d(G-C)] and poly[d(A-C) · d(G-T)] families of helices have been determined. The specificities of the resultant immunoglobulins have been characterized for recognition of different synthetic and natural left-handed sequences and conformations. Certain modifications of poly[d(G-C)] in the sugar-phosphate bacbone and cytosine C-5 potentiate the right(R)-to-left(L) (B → Z) transition under physiological conditions. The resulting polynucleotides, poly[d(GS-C)], poly[d(G-io5C)], poly[d(G-br5C)] and poly[d(G-m5C)], are also highly immunogenic. In contrast, DNAs incapable of assuming the left-handed conformation under physiological salt concentrations are weakly or non-immunogenic. These include unmodified poly[d(G-C)] as well as members of the poly[d(A-C) · d(G-T)] family of sequences bearing pyrimidine C-5 substitutions (methyl, bromo, iodo). These polynucleotides undergo the R → L isomerization under more stringent ionic and thermal conditions.The specificities of purified polyclonal and monoclonal anti-Z DNA immunoglobulins (IgG) were measured by binding to radiolabeled polynucleotides, by electrophoretic analysis of IgG bound to covalent closed circular DNAs, and by immunofluorescent staining of polytene chromosomes. The salt-induced left-handed forms of poly[d(G-C)] and its derivatives (including the cytidine C-5 methyl, bromo, iodo, and N-5 aza substituted polynucleotides) and of the modified poly[d(A-C) · d(G-T)] polymers are bound to varying degrees by different antibodies. The patterns of substrate recognition demonstrate the existence of several antigenic domains in left-handed DNAs, including the helix convex surface and the sugar-phosphate backbone. Substitutions in these regions can produce enhancing (required substitutions), neutral, or inhibitory effects on subsequent IgG binding. Additionally, certain modifications of either the convex surface of Z DNA at the C-5 position of cytidine (i.e. a methyl group) or of the backbone (i.e. phosphorothioate substitution) can lead to polymorphic lefthanded conformations that are compatible with antibody binding when present individually but not in combination. The recognition patterns exhibited with DNA substrates from the two DNA families indicate that some, but not all, IgGs show specificity for different nucleotide sequences.The anti-Z DNA IgGs were used to probe for specific left-handed Z DNA determinants on plasmid (e.g. pBR322) or viral (e.g. simian virus 40 (SV40)) DNAs and on the acid-fixed polytene chromosomes of dipteran larvae. At their extracted superhelical density, the negatively supercoiled form I, but not the relaxed, nicked, or linear forms of all tested plasmid and viral DNAs specifically bind sequence-independent anti-Z IgGs. Dimers, trimers and higher oligomers of form I DNA cross-linked by bivalent anti-Z IgGs are formed with numerous (e.g. φX174, SV40, pBR322) genomes. Their occurrence depends upon IgG concentration and specificity, the conditions of ionic strength and temperatures and the DNA genome. The IgG cross-linked DNA multimers are converted to monomers by dithiothreitol reduction. Sequence-independent monovalent anti-Z Fab fragments bind form I DNA but do not generate oligomeric species. Multimers of order >2 indicate the existence of at least two anti-Z Ig binding sites per molecule, as in the case of SV40. IgGs differ in their ability to form stable complexes with some sites on natural DNAs, presumably due to their sequence and conformation binding specificities. A differential binding of these antibodies is also observed in certain bands of polytene chromosomes, such as the telomeric regions that are involved in chromosome associations. 相似文献
35.
36.
John Richard Seed 《International journal for parasitology》1977,7(1):55-60
The effects of IgM and IgG antibody molecules were compared on a weight basis by both agglutination and in vitro protection tests. It was shown that IgM is a better agglutinating antibody and in the presence of complement is also a better neutralizing antibody. However, when IgM and IgG were tested for their ability to passively protect infected animals, it was noted that the IgG fraction appeared to give greater protection. Based on differences in diffusion coefficients (and size) of the molecules, it is hypothesized that IgM is the antibody class responsible for the relapse phenomena observed in the blood, while, it is the IgG antibody molecule which is more active in extravascular locations. 相似文献
37.
38.
Antibodies against Nippostrongylus brasiliensis were demonstrated by the indirect fluorescent antibody technique in four pools of sera from mice 3 weeks after one or more exposures to this parasite. These antibodies combined with antigens in sections of N. brasiliensis and included IgG, IgM, and IgA classes of immunoglobulins. Antibodies of the first two classes produced intense fluorescence in many areas of the parasites, whereas IgA usually evoked only minimal reactions at most of these same sites. Results produced by all pools of antisera were similar, while pools of sera from nonparasitized mice were essentially negative.The principal site of fluorescence in sections treated with antisera was in the cellular cytoplasm and in the microvillar layer of the intestinal epithelium. The nuclei in these cells did not fluoresce. The cuticle, lateral canals, body wall musculature, and reproductive organs fluoresced to a lesser extent. In this group of structures, the most notable fluorescence occurred in the cytoplasm of developing ova, in shells of completed eggs, and in muscle cells of the vagina. Slight autofluorescence was observed in the cuticle, cytoplasm of cells of the lateral canals, substances in the lumina of the lateral canals, and in the extracellular substance of the excretory glands. 相似文献
39.
Kushimo J. B. and Akinrimisi E. O. Immune response to deoxyribonucleic acid (DNA) of African trypanosomes. International Journal for Parasitology12: 537–540. Rabbits immunized with methylated bovine serum albumin (MBSA) complexes of nuclear DNA from either T. brucei or T. vivax which have low content of Adenine + Thymine (A + T) produced only IgM antibodies to denatured DNA. On the other hand rabbits immunized with MBSA complexes of denatured kinetoplast DNA (K-DNA) from either T. brucei or T. vivax which are rich in A + T content elicit both IgM and IgG antibodies. However the amount of IgG antibodies was higher than IgM antibodies. There seems to be a correlation between % AT content of immunogen and average ratio of maximum precipitable IgG to IgM (IgG)/(IgM). 相似文献
40.
目的分析麻疹疑似病例血清学和病原学的检测结果,比较两种检测方法,为麻疹的早期诊断提供实验室支持。方法同时采集2017-2018年北京市海淀区麻疹疑似病例的血清和咽拭子标本,用酶联免疫吸附试验(ELISA)方法检测血清中的麻疹IgM抗体,用荧光定量PCR(Real-time PCR)方法检测咽拭子标本中的麻疹病毒核酸。结果血清IgM抗体检测阳性率为11.54%,Real-time PCR法检测阳性率为44.23%,其检测阳性率显著高于血清检测阳性率,差异有统计学意义(χ~2=13.82,P0.01)。ELISA方法在出疹3 d内采集的阳性率为12.77%,Real-time PCR方法的阳性率为53.85%,差异有统计学意义(χ~2=16.70,P0.01);ELISA方法在出疹3 d后采集的阳性率为0.00%,Real-time PCR方法的阳性率为15.38%,二者比较差异无统计学意义(P0.05)。血清学检测敏感性为25.00%,病原学检测敏感性为95.83%,两种检测方法的阳性符合率为21.74%,阴性符合率为96.55%,总符合率为63.46%。ELISA和Real-time PCR法对有免疫史的病例检测阳性率分别为18.75%和37.50%,两种检测方法的阳性率差异无统计学意义(χ~2=1.39,P0.05);对无免疫史或免疫史不详病例检测的阳性率分别为8.30%和47.20%,两种检测方法的阳性率差异有统计学意义(χ~2=13.57,P0.01)。结论 Real-time PCR方法检测的阳性率和灵敏度均高于血清学检测方法,可以在日常检测工作中作为常规方法推广,无论采用哪种检测方法,应在出疹3 d内采集样本。 相似文献