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71.
Mauro S. Sandrin Hilary A. Vaughan Ian F. C. McKenzie Brian D. Tait Christopher R. Parish 《Immunogenetics》1979,8(1):185-200
The production of xenogeneic anti-Ia serum against Ia antigens in serum has been previously described in the mouse and we now describe the production of xenogeneic anti-human Ia antisera using similar methods. With an indirect resetting technique, Ia-like antibodies were shown to react with the majority of B cells (95%), a subpopulation of T cells, with carbonyl iron adherent cells, and with some E–Ig– null cells, but there was no reaction with red cells and platelets. These reactions were the same as those obtained with DRW antisera using cytotoxicity testing. In addition, antigens detected with xenogeneic antisera were also found in serum, where they were found to exist in a low molecular weight, dialyzable form. By the selective removal of different cell surface markers by cocapping, no association could be found with the specifities detected with the xenogeneic anti-Ia antisera and with surface Ig,
2-microglobulin, or HLA-A and B specificities. Alloantibodies to DRW specificities (but not HLA-A, B specificities) were able to specifically block the binding of the rabbit anti-Ia antibodies to B cells, and reciprocal blocking of rabbit antisera by DRW antibodies was also observed. Several xenogenic antisera were produced by immunizing rabbits with the serum of different individuals. Each antiserum was shown to contain a number of different specificities, as they gave different reaction patterns with different individuals when testing was done both directly and by absorption. These xenogeneic anti-la sera also segregated in a family with HLA-A and B specificities. The detection of a polymorphic antigenic system segregating with the HLA complex, distinct from HLA-A and B specificities, and whose antigens occur predominantly on B cells is therefore described. Because of the similarity of the reactions of the xenogeneic antisera in man to those found in the mouse, and because of the close relationship to the DRW specificities, the system has been provisionally called the H.Ia system.Abbreviations used in this paper AET
2-aminoethyl isothiouronium bromide
-
2-M
-2 microglobulin
- BSA
Bovine serum albumin
- H.Ia
Human Ia
- HuRBC
Human red blood cells
- Ig
Immunoglobulin
- Ir
Immune response
- MHC
Major histocompatibility complex
- MLR
Mixed lymphocyte reaction
- NHS
Normal human serum
- NMS
Normal mouse serum
- PBL
Peripheral blood lymphocytes
- PBS
Phosphate-buffered saline
- RAHIg
Rabbit anti-human immunoglobulin
- RASIg
Rabbit anti-sheep immunoglobulin
- RFC
Rosette-forming cells
- SAHIg
Sheep anti-human immunoglobulin
- SARIy
Sheep anti-rabbit immunoglobulin
- SRBC
Sheep red blood cells 相似文献
72.
J H Barber D G Beevers R Fife V M Hawthorne H M McKenzie R G Sinclair R J Simpson G M Stewart D I Williams 《BMJ (Clinical research ed.)》1979,1(6167):843-846
Since April 1975 all men aged 35-69 years registered with four general practices in west central Scotland have had their blood pressure checked whenever they visit the surgery. Although the practice locations range from rural to city centre and observers comprise receptionists, nurses, and doctors, a standard procedure has been adopted for the examination, recording, follow-up, and management of high blood pressure. The results confirm that raised blood pressure is common and often goes undetected. Even when hypertension is known, casual blood pressure readings often exceed accepted normal levels. The findings also show that a population may be routinely examined through normal contact with the family doctor, and that this can provide a convenient, acceptable, and effective means of detecting and reducing raised blood pressure. 相似文献
73.
Irradiated CBA anti-DBA/2 cells (106 cells/culture) suppressed the production of effector cells in cultures containing 107 unprimed CBA (responder) and 106 irradiated DBA/2 (stimulator) spleen cells per culture. The suppressive element was cellular and suppression was specific for the stimulating antigen. The suppressive activity resided in the cytotoxic cell population in that both suppressive and cytotoxic activities were found in cells of the same size range, predominantly in T-cells, were produced in response to similar doses of stimulator antigen, and were produced with the same time course following establishment of first sensitization cultures. Eventual suppression correlated with the cytotoxic activity introduced into second sensitization cultures by suppressor cells. The short-term cytotoxic activity and suppressor activity were both highly radioresistant. These studies indicate that the suppressor cells formed in an in vitro mixed lymphocyte culture are cytotoxic to stimulator cells. 相似文献
74.
75.
76.
William McKenzie 《BMJ (Clinical research ed.)》1962,2(5320):1680-1681
77.
78.
79.
Katrina Laks Tiina Kirsipuu Tuuli Dmitrijeva Andres Salumets Peep Palumaa 《The protein journal》2016,35(3):171-176
Biological fluid sample collection often includes the risk of blood contamination that may alter the proteomic profile of biological fluid. In proteomics studies, exclusion of contaminated samples is usually based on visual inspection and counting of red blood cells in the sample; analysis of specific blood derived proteins is less used. To fill the gap, we developed a fast and sensitive method for ascertainment of blood contamination in crude biological fluids, based on specific blood-derived protein, hemoglobin detection by MALDI-TOF MS. The MALDI-TOF MS based method allows detection of trace hemoglobin with the detection limit of 0.12 nM. UV-spectrometry, which was used as reference method, was found to be less sensitive. The main advantages of the presented method are that it is fast, effective, sensitive, requires very small sample amount and can be applied for detection of blood contamination in various biological fluids collected for proteomics studies. Method applicability was tested on human cerebrospinal and follicular fluid, which proteomes generally do not contain hemoglobin, however, which possess high risk for blood contamination. Present method successfully detected the blood contamination in 12 % of cerebrospinal fluid and 24 % of follicular fluid samples. High percentage of contaminated samples accentuates the need for initial inspection of proteomic samples to avoid incorrect results from blood proteome overlap. 相似文献
80.