| ²é¿´: 845 | »Ø¸´: 2 | |||
| µ±Ç°Ö÷ÌâÒѾ´æµµ¡£ | |||
| µ±Ç°Ö»ÏÔʾÂú×ãÖ¸¶¨Ìõ¼þµÄ»ØÌû£¬µã»÷ÕâÀï²é¿´±¾»°ÌâµÄËùÓлØÌû | |||
china-dragonľ³æ (ÕýʽдÊÖ)
|
[½»Á÷]
ÁÙ´²¼ìÑé
|
||
|
ÁÙ´²¼ìÑé BÁÜ°Íϸ°û B lymphocyte TÁÜ°Íϸ°û T lymphocyte °¬µÏ˹¼ÆÊý Addis count °×ϸ°û leucocyte, white blood cell, WBC °×ϸ°û·ÖÀà¼ÆÊý white blood cell differential count, leucocyte differential count °×ϸ°û¹ÜÐÍ leucocyte cast, white blood cell cast °×ϸ°ûÄò leucocyturia °ØÓÍÑù±ã tarry stool ±¾Öܵ°°× Bence-Jones protein ²£Æ¬£¬ÔØƬ slide ²»µäÐÍÁÜ°Íϸ°û atypical lymphocyte ²ÝËá¸Æ½á¾§ crystals of calcium oxalate ³öѪʱ¼ä bleeding time, BT µ¥ºËϸ°û monocyte, MO, mononuclear leucocyte µ¨ºìËØÄò bilirubinuria µ¨ÄÒÒýÁ÷Òº cholecyst drainage solution µ°°×Äò proteinuria, albuminuria, serumuria ¶þ¼×±½ xylol ·Æʲ²®¸ñŨËõÊÔÑé Fishberg concentration test ·ÓºìÅÅйÊÔÑé phenolsulfonphthalein excretion test ·à±ã stool, feces, excrement ·à±ã³£¹æ¼ì²é stool routine test ·à±ãŨ¼¯·¨²é³æÂÑ fecal ova by concentrated method ·à±ãDZѪÊÔÑé stool occult blood test ·à±ãͿƬ·¨²é³æÂÑ fecal ova by smear method ·à±ãÐÔ×´ characteristics of feces ·à±ãÔ³æ¼ø¶¨ identification of protozoa in feces ·à±ãÖ¬·¾ fats in feces ·àß²ßø coproporphyrin, stercoporphyrin ·àµ¨ËØ stercobilin ·àµ¨ËØÔ stercobilinogen ·àʯ fecalith, coprolith, stercolith ¸ßÌúºìϸ°ûȾɫ·¨ siderocyte staining ¸ßÌúѪºìµ°°× methemoglobin ¸ßÌúѪºìµ°°×Ѫ֢ methemoglobinemia ¹ÇËè bone marrow ¹ÇËèϸ°û·ÖÀà¼ÆÊý differential count of bone marrow cells ºì°ßÀÇ´¯Ï¸°û lupus erythematosus cell,LEC ºì°ßÀÇ´¯ÏÖÏó lupus erythematosus phenomenon ºìϸ°û erythrocyte, red blood cell, RBC ºìϸ°û³Á½µÂÊ erythrocyte sedimentation rate, ESR ºìϸ°ûµçÓ¾ erythrocyte electrophoresis ºìϸ°û¹ÜÐÍ red blood cell cast ºìϸ°û¼ÆÊý erythrocyte count ºìϸ°ûƽ¾ùÌå»ý mean corpuscular volume, MCV ºìϸ°ûƽ¾ùѪºìµ°°×Á¿ mean corpuscular hemoglobin, MCH ºìϸ°ûƽ¾ùѪºìµ°°×Ũ¶È mean corpuscular hemoglobin concentration, MCHC ºìϸ°ûÌå»ý·Ö²¼¿í¶È red cell volume distribution width, RDW »ìѪøÔʱ¼ä prothrombin time, PT »î»¯µÄ²¿·ÖÄýѪ»îøʱ¼ä activated partial thromboplastin time, APTT ¼ªÄ·ÈøȾɫ·¨ Giemsa's staining ¼ÄÉú³æ parasite ¼äÖÊϸ°û mesenchymal cell, mesothelial cell ½¬Ä¤Ç»Òº serous cavity fluid, serow membrane effusion ½¬Ï¸°û plasma cell ¾«Òº semina, sperm, semen ¾«Òº³£¹æ¼ì²é semen routine examination ¾«ÒºÄò spermaturia, semenuria ¾«×Ó sperm, spermatozoon, spermatoblast ¾«×Ó´æ»îÂÊ sperm survival rate ¾«×Ó»îÁ¦ sperm activity ¾«×Ó»îÁ¦²»×ã asthenospermia ÎÞ¾«×ÓÖ¢ azoospermia, azoospermatism ¾«×Ó¼ÆÊý sperm count ¾«×Óȱ·¦£¬¾«×Ó¹ýÉÙ spermacrasia ¾«×ÓÈܽâ spermatolysis ¾«×ÓÐÎ̬ѧ sperm morphology ¾ÞÊÉϸ°û macrophage ¿ÅÁ£¹ÜÐÍ granular cast À¯Ñù¹ÜÐÎ waxy cast ÀïÍ߶ûËþ·´Ó¦ Rivalta reaction Á£Ï¸°û granulocyte Á×´ºìϸ°û sickle erythrocyte ÁÜ°Íϸ°û lymphocyte ÁÜ°Íϸ°ûÑÇȺ·ÖÀà differential of lymphocyte subpopulation ©³öÒº transudate ë·¢ hair, pilus Ä¿¾µ ocular Ä¿¾µ²â΢¼Æ ocular micrometer ÄÔ¼¹Òº³£¹æ¼ì²é cerebrospinal fluid routine examination ÄÔ¼¹Òºµ°°×¶¨ÐÔ qualitative test for cerebrospinal fluid protein ÄòpH urine pH Äò°ëÈéÌǶ¨ÐÔÊÔÑé qualitative test for urinary galactose Äò±½±ûͪËá²â¶¨ determination of urinary phenylpyruvic acid Äò±ÈÃܲâÁ¿·¨ urinometry, determination of urine specific gravity Äòß²ßø¶¨Á¿ÊÔÑé quantitative test for uroporphyrin Äòß²ßø¶¨ÐÔÊÔÑé qualitative test for uroporphyrin Äò³£¹æ¼ì²é urine routine test, routine urinalysis Äò³ÁÔü¾µ¼ì microscopic examination of urinary sediment Äòµ¨ºìËض¨ÐÔÊÔÑé qualitative test for urinary bilirubin Äòµ¨ºìËØÊÔÑé urinary bilirubin test, urobilirubin test Äòµ¨É«ËØÔ¶¨ÐÔÊÔÑé qualitative test for porphobilinogen Äòµ¨ËØ urobilin Äòµ¨ËØÔ£¬Äòµ¨Ô urobilinogen Äòµ°°×¶¨Á¿ÊÔÑé quantitative test for urinary protein Äòµ°°×¶¨ÐÔÊÔÑé qualitative test for urinary protein Äò¸Æ¶¨ÐÔ¼ì²é qualitative test for urinary calcium Äò¹ûÌǶ¨ÐÔÊÔÑé qualitative test for urinary fructose ÄòŨËõÊÔÑé urine concentration test ÄòDZѪÊÔÑé urinary occult blood test ÄòÈܾúø lysozyme in urine ÄòÈéÌǶ¨ÐÔÊÔÑé qualitative test for urinary lactose ÄòÌǶ¨Á¿ÊÔÑé quantitative test for urinary glucose ÄòÌǶ¨ÐÔÊÔÑé qualitative test for urinary glucose ÄòÌÇÊÔÑé urinary glucose test ÄòͪÌå urinary ketone bodies ÄòÑÇÏõËáÑÎÊÔÑé urinary nitrite test ÄòÒº·ÖÎö urine analysis, urinalysis ÄýѪø thrombin, thrombase ÄýѪøʱ¼ä thrombin time, TT ÄýÑªÃ¸Ô prothrombin ÄýѪʱ¼ä clotting time, CT űԳæ malarial parasite, plasmodium Ƥ·ô skin ȫѪ¼ÆÊý complete blood count, CBC ÈéÃÓÄò chyluria, galacturia ÈéÃÓѪ chylaemia ÈðÊÏȾɫ·¨ Wright's staining É«°±ËáÊÔÑé tryptophan test Éø³öÒº exudate Ê®¶þÖ¸³¦Òº duodenal juice ÊȼîÐÔÁ£Ï¸°û basophil, BA, basophilic leucocyte ÊÈËáÐÔÁ£Ï¸°û eosinophil, EOS ÊÈËáÐÔÁ£Ï¸°ûÖ±½Ó¼ÆÊý direct count for eosinophil ÊÈËáÐÔϸ°û¼õÉÙ eosinopenia ÊÈËáÐÔϸ°ûÔö¶à eosinophilia Ë¿³æ¼ì²é examination of filaria ËÕµ¤ºÚBȾɫ·¨ Sudan black B staining ËữѪÇåÊÔÑé acidified serum test ̼ÑõѪºìµ°°×Ѫ֢,Ò»Ñõ»¯Ì¼Öж¾ carboxyhemoglobinemia ͸Ã÷¹ÜÐÍ hyaline cast ͿƬ£¬Ä¨ smear ÍøÖ¯ºìϸ°û reticulocyte θҺ gastric juice θҺ·ÖÎö gastric juice analysis ÎÂ¶È temperature ÎÂ¶È¼Æ thermometer ϸ°û¹ÜÐÍ cellular cast ϸ°ûºË£¬ºË caryon, kernel, nucleus ÏÔ΢¾µ microscope Ѫ£¨Äý£©¿é blood clot Ѫ³£¹æ¼ì²é blood routine examination, routine examination of blood Ѫºìµ°°× hemoglobin, Hb Ѫºìµ°°×µçÓ¾ hemoglobin electrophoresis Ѫºìµ°°×¹ÜÐÍ hemoglobin cast ѪºìËØ heme Ѫ¿â blood bank Ѫ¿éÄýËõʱ¼ä clot retraction time, CRT ѪÄý¹Ì hemopexis, blood coagulation ѪɫËØ hemochrome, hematochrome Ѫϸ°û hemacyte, hemocyte, blood cell Ѫϸ°û±ÈÈÝ hematocrit, HCT£¬£¨ packed cell volume£© ¾É³Æºìϸ°ûѹ»ý£¬ Ѫϸ°û¼ÆÊý blood count, cytometry Ѫϸ°û¼ÆÊý³Ø blood counting chamber Ѫϸ°û¼ÆÊý·¨ hemacytometry, hemocytometry,hematimetry Ѫϸ°û¼ÆÊýÆ÷ cytometer, hemocytometer, hematimeter ѪÏñ hemogram ѪС°å±ÈÈÝ plateletcrit, PCT ѪС°å»î»¯Òò×Ó platelet activating factor, PAF ѪС°å¾Û¼¯ÊÔÑé platelet aggregation test ѪС°åƽ¾ùÌå»ý mean platelet volume, MPV ѪС°åÌå»ý·Ö²¼¿í¶È platelet volume distribution width, PDW ѪС°åÕ³¸½ÊÔÑé platelet adhesion test ѪÐÍ blood group, blood type ѪÐͲ»ºÏ blood group incompatibility ѪÐͼø¶¨ determination of blood group, blood grouping ѪÐÔ¸¹Ë® bloody ascites, sanguineous ascites ѪÐÔ¾«Òº hematospermia, hemospermia ѪҺ±ê±¾ blood specimen ѪҺѧ hematology ѪҺѧ¼ì²é hematological examination ѪҺÑùÆ· blood sample ѪҺճ¶È²â¶¨ determination of blood viscosity Òì³£ºìϸ°ûÐÎ̬ abnormal erythrocyte morphology Óͽþ¾µ oil immersion lens ÓÎÀëËá¶È free acidity Óк˺ìϸ°û nucleated erythrocyte Ó×µ¥ºËϸ°û juvenile monocyte Ó×ÁÜ°Íϸ°û juvenile lymphocyte Ó×ÖÉϸ°û juvenile cell ÔÉúÖÊ protoplasm(bioplasm) ÔçÓ×Á£Ï¸°û promyelocyte Õ³Òº mucus ÕáÌÇÈÜѪÊÔÑé sucrose lysis test, sucrose hemolysis test ÖÐÐÔ·ÖÒ¶ºË°×ϸ°û neutrophil segmented gronulocyte ÖÐÐÔ¸Ë×´ºËÁ£Ï¸°û neutrophil stab(band) granulocyte ÖÐÐÔÁ£Ï¸°û neutrophil graneulocyte ÖÐÐÔÁ£Ï¸°û°Ù·ÖÊý neutrophil percent, NE% ÖÐÐÔÁ£Ï¸°ûÊý neutrophil number, NE ÖÐÐÔÍíÓ×Á£Ï¸°û neutrophilic metamyelocyte ÖÐÐÔÖÐÓ×Á£Ï¸°û neutrophil myelocyte ×ÜËá¶È total acidity |
»Ø¸´´ËÂ¥» ²ÂÄãϲ»¶
³£ÓÃÖ×Áö¶¯ÎïÄ£Ð͵Ĺ¹½¨
ÒѾÓÐ0È˻ظ´
-
´óÊó¹àθÑÛ¾¦×ì°Í³öѪʲôÔÒò
ÒѾÓÐ1È˻ظ´
-
Ô˶¯ÏµÍ³ÂÛÎÄÈóÉ«/·ÒëÔõôÊÕ·Ñ?
ÒѾÓÐ181È˻ظ´
-
ÖÐҩѧ
ÒѾÓÐ0È˻ظ´
-
ÇóÖúÒ©Àí·½Ïò¹¤×÷Á¿ÉÙÄÜͶʲô˫ºË£¿
ÒѾÓÐ1È˻ظ´
-
ÂÌÔËá¶ÔÕÕÈÜÒºÅäÖÆ1¸öÔ£¬ÅäÍêÖ®ºóÒ»Ö±·Å±ùÏ䣬ÏÖÔÚ·åÃæ»ýµÍÁË30£¬»á½µ½âÕâô¿ìÂð
ÒѾÓÐ3È˻ظ´
-
5/6ÉöÇгýÔìÂýÐÔÉöÔ༲²¡£¬²¿·ÖÇгýµÄ²ÐÉöÓëÖ¬·¾Õ³Á¬£¬Õâ¸öÕý³£Âð£¿
ÒѾÓÐ0È˻ظ´
-
Î÷Ò½ 306 ר˶һ־Ը b Çø
ÒѾÓÐ9È˻ظ´
china-dragon
ľ³æ (ÕýʽдÊÖ)
- Ó¦Öú: 0 (Ó׶ùÔ°)
- ½ð±Ò: 2961
- Ìû×Ó: 425
- ÔÚÏß: 14.3Сʱ
- ³æºÅ: 247034
- ×¢²á: 2006-04-30
- רҵ: ÁÙ´²ÉúÎﻯѧ¼ìÑé
|
ÉöËØ renin ÉöÌÇãÐ renal glucose threshold Éø͸ÈÜÖÊ osmolute Éø͸ѹ¼Æ osmometer Éú³¤¼¤ËØ growth hormone ÉúÎï·¢¹â bioluminescence ÉúÎïÀûÓÃÂÊ bioavailability ÉúÎïоƬ Bio-Chip ʪ»¯Ñ§ wet chemistry ʯµ¨Ëá lithocholic acid ʯī¯ graphite furnace ʱ¼ä·Ö±æÓ«¹â¼Æ time resolved fluorometer ʵ¼Ê¼î¹ýÊ£ actual bicarbonate excess ʵ¼Ê̼ËáÇâÑÎ actual bicarbonate, AB Êӻƴ¼½áºÏµ°°× retinol-binding protein, RBP ÊÔ¼Á¼¶ reagent grade Ê÷Ö¬·¨ resin method Ë«²¨³¤·Ö¹â¹â¶È²â¶¨·¨ dual wavelength spectrophotometry Ë«ÆÏÌÑÌÇÈ©ËᵨºìËØ bilirubin diglucuronide ¼´Ë«ÆÏÌÑÌÇÈ©Ëáõ¥ Ë«Ëõëå·¨ biuret method ˳Ðò·ÖÎöÒÇ sequential analyzer ËÙÂÊ·¨ kinetic rate method ËáÐÔÁ×Ëáø acid phosphatase, ACP ôÈ»ùÄ©¶Ë C-terminal Óֳơ°CÄ©¶Ë¡± ̨ʽÀëÐÄ»ú bench-top centrifuge ̼ˮ»¯ºÏÎï carbohydrate Óֳơ°ÌÇÀࡱ ̼Ëáôûø carbonic anhydrase ÌÇ»¯Ñªºìµ°°× glycosylated hemoglobin, GHb ÌÇ»¯ÑªÇåµ°°× glycosylated serum protein, GSP Ìǽͽâ×÷Óà glycolysis ÌÇƤÖʼ¤ËØ glucocorticoid ͬ¹¤Ã¸ isoenzyme, isozyme ͬ루ºË£©ËØÏ¡ÊÍÖÊÆ×·ÖÎö isotope-dilution mass spectrometry ͬÐÍ°ëë×°±Ëᣬ¸ß°ëë×°±Ëá homocysteine, HCY Í copper ͸¹â¶È transmittance ͸Éä±È×Ç·¨ turbidimetry ÍÐ torr ¾ÉÆøÌåѹÁ¦µ¥Î» ÍÑÑõµ¨Ëá deoxycholic acid ΢Á¿ÔªËØ trace element, minim element ÎÈ̬ steady state ÎÞµ°°×ÂËÒº protein free filtrate ÎÞÑæÔ×ÓÎüÊÕ flameless atomic absorption ÎÞÑõ´¦Àí anaerobic handling Óֳơ°ÑáÑõ´¦Àí¡± ÎìÌÇÄò pentosuria Îü¹â¶È absorbance ÎüÊÕ³Ø absorption cell Óֳơ°±ÈÉ«±¡± ÎüÊÕ¹âÆ× absorption spectrum ÎüÊÕϵÊý absorption coefficient ÎüÊÕÏà sabsorption phase Ï¡ÊÍÆ÷ dilutor ϳÁÇ°¦ÂÖ¬µ°°× sinking pre ¦Â-lipoprotein ÏËάµ°°×Ô fibrinogen õ£»ù¸¨Ã¸Aµ¨¹Ì´¼õ£»ùתÒÆø acylCoA: cholesterol acyltransferase, ACAT õ£»ù¸ÊÓÍ acylglycerol Óֳơ°¸ÊÓÍõ¥¡±¡£ Ïß·¢Éä line emission, line emitting ÏÙÜÕÍÑ°±Ã¸ adenosine deaminase, ADA Ïà¶ÔÀëÐÄÁ¦ relative centrifugal force, RCF Ïã²Ý±âÌÒËᣬ3-ÂÈ-4-ôÇÐÓÈÊËá vanillylmandelic acid, VMA Ïû³ý°ëÊÙÆÚ half life of elimination Ïû³ýÏà elimination phase ÐÄ°üÒº£¬ÐÄ°ü»ýÒº pericardial fluid ÐÄ·¿ÄÆÄòëÄ atrial natriuretic peptide, ANP Óֳơ°ÐÄÄÆËØ£¬ÐÄ·¿ëÄ¡±¡£ Ðļ¡¼¡¸Æµ°°×I cardial troponin I, cTnI Ðļ¡¼¡¸Æµ°°×T cardiac troponin T, cTnT п zinc ÐØË® pleural fluid ÐÛ¼¤ËØ antrogen ÐÜÍÑÑõµ¨Ëá ursodeoxycholic acid äå¼×·ÓÂÌ bromocresol green, BCG Ѫ°±²â¶¨ blood ammonia determination Ѫ¹Ü½ôÕÅËØ angiotensin Óֳơ°Ñª¹Ü½ôÕÅëÄ¡± Ѫ¹Ü½ôÕÅËØת»¯Ã¸ angiotensin converting enzyme, ACE Ѫºìµ°°×A1C hemoglobin A1C, HbA1c Ѫ½¬ÍÀ¶µ°°× ceruloplasmi, CP ѪÆø·ÖÎö blood gas analysis ѪÇåµ°°× serum protein Ѫ˨Íé thromboxane Óֳơ°ÑªË¨ËØ¡± ѪÌDZ£´æ¼Á preservative for blood glucose Ñ֤ҽѧ evidence-based medicime, EBM ÑÌõ£°·ÏÙàÑßʶþºËÜÕËá nicotinamide adenine dinucleotide, NAD Óֳơ°¸¨Ã¸I¡± ÑÌõ£°·ÏÙàÑßʶþºËÜÕËáÁ×Ëá nicotinamide adenine dinucleotide phosphate, NADP Óֳơ°¸¨Ã¸II¡± ÑÎƤÖʼ¤ËØ mineralocorticoid ÑÎÎö salting out ÑòË® amniotic fluid Ñõ±¥ºÍ[¶È] oxygen saturation,O2 saturation, O2Sat Ñõ·Öѹ partial pressure of oxygen, pappenheimer O2, PO2 Ñõº¬Á¿ oxygen content, O2 cont ÑõºÏѪºìµ°°×½âÀëÇúÏß oxyhemoglobin dissociation curve Ñõ»¯îز£Á§ holmium oxide glass Ñõ½áºÏÁ¦ oxygen capacity Ò»´ÎÐÔʹÓõģ¬Ò×´¦ÖÃµÄ disposable Ò»¼¶´úл first order metabolism Ò»¼¶·´Ó¦ first order reaction Òȵ°°×ø trypsin, trypsinase ÒȵºËØ insulin ÒȸßѪÌÇËØ glucagon Òƶ¯½çÃæµçÓ¾ moving boundary electrophoresis Óֳơ°ÒƽçµçÓ¾¡±¡£ ÒÆÒº¹Ü pipet ÒÒËáÏËάËØ acetate cellulose ÒõÀë×Ó϶ anion gap, AG Ó«¹â²â¶¨·¨ fluorometry Ó«¹â·Ö¹â¹â¶È¼Æ spectrofluorimeter Ó«¹âÆ«Õñ·ÖÎö fluorescence polarization analysis ÓªÑøËØ£¬ÓªÑøÎï nutrient ÓÎÀ뵨¹Ì´¼ free cholesterol ÓÎÀë¸ÊÓÍ free glycerol ÓÎÀë¼××´ÏÙËØ free thyroxine, FT4 ÓÎÀë¼××´ÏÙËØÖ¸Êý free thyroxine index, FTI ÓÎÀëÈýµâ¼×ÏÙÔ°±Ëá free triiodothyronine, FT3 Ô×ÓÎüÊÕ·Ö¹â¹â¶È¼Æ stomic absorption spectrophotometer ÔȽ¬Æ÷ homogenizer Ôжþ´¼ pregnanediol ÔÐÈý´¼ pregnanetriol ÔÐͪ progesterone ÔØÖ¬µ°°× apolipoprotein Ôí»¯£¨×÷Óã© saponification Õ³µ°°×²â¶¨ mucoprotein determination, Rivalta test ÕÅÁ¦²âÁ¿·¨ tonometry Óֳơ°Ñ¹Á¦²âÁ¿·¨¡± Õæ¿Õ²ÉѪ¹Ü evacuated blood tube Õæ¿Õ¸ÉÔïÆ÷ vacuum desiccator ÕæÖµ true value Ö¬µ°°× lipoprotein Ö¬µ°°×£¨a£© lipoprotein (a), Lp(a) Ö¬µ°°×ÊÜÌå lipoprotein receptor Ö¬µ°°×Ö¬·¾Ã¸ lipoprotein lipase, LPL Ö¬·¾Ã¸ lipase, LPS; LIP Ö¬·¾Ëá fatty acid Ö¬·¾Ëá½áºÏµ°°× fatty acid binding protein, FABP Ö¬À࣬֬ÖÊ lipid Ö¬ÀàתÔ˵°°× lipid transfer protein Óֳơ°Ö¬ÖÊתÔ˵°°×¡± Ö¬ÖʹýÑõ»¯×÷Óà lipid peroxidation ÖÊÁ¿Å¨¶È mass concentration ÖÊÆ×·ÖÎö mass spectrometry ÖмäÃܶÈÖ¬µ°°× intermediate density lipoprotein, IDL ÖÐÐÔÖ¬·¾ neutral fat ÖÐ×ӻ·ÖÎö neutron activation analysis Öյ㷨 end-point method ÖØ£¨ÖØÁ¿£© weight, WT ÖصªÊÔ¼Á diazo reagent ÖØÁ¿Ä¦¶ûŨ¶È molality ÖØÁ¿Éø͸Ħ¶ûŨ¶È osmolality Óֳơ°ÖØÁ¿¿Ë·Ö×ÓŨ¶È¡±¡£ ÈÝÁ¿Éø͸Ħ¶ûŨ¶È osmolarity Óֳơ°ÈÝ»ýÉø¿Ë·Ö×ÓŨ¶È¡± תÒƵçÓ¾ transfer electrophoresis ׼ȷ¶È accuracy ×ܵ¨¹Ì´¼ total cholesterol, TC ×ܵ¨ºìËØ total bilirubin ×ܵ¨ÖËá total bile acid, TBA ×ܵ°°× total protein ×ܶþÑõ»¯Ì¼£¬¶þÑõ»¯Ì¼×ÜÁ¿ total CO2, TCO2 ×î´óÎüÊÕ maximum absorption ¼¡ºìµ°°× myoglobin£¬Myo,Mb ´Æ¼¤ËØÊÜÌå estrogen recepter,ER ÄÚƤËØ endothelin,ET Ì¥¶ùÏËάÁ¬½Óµ°°× fetal fibronectin,Ffin ´ÙÐÔÏÙ¼¤ËØ gonadotropin,Gn ´ÙÐÔÏÙ¼¤ËØÊͷż¤ËØ gonadotropin releasing hormone,Gn-RH £¨ÈË£©¾ø¾ÆÚ´ÙÐÔÏÙ¼¤ËØ human menopausal gonadotropin,HMG £¨ÈË£©Ì¥ÅÌÉúÈéËØ human placental lactogen,HPL ÂÑÁ×Ö¬/ÇÊÁ×Ö¬ lacithin/sphingomyelin,L/S Ç°ÁÐÏÙËØE prostaglandin E,PGE Ç°ÁÐÏÙËØF2¦Á prostaglandin F2¦Á£¬PGF2¦Á Ôм¤ËØÊÜÌå progenstogen receptor,PR ´ßÈ鼤ËØ prolactin,PRL |
3Â¥2006-05-09 19:20:32
china-dragon
ľ³æ (ÕýʽдÊÖ)
- Ó¦Öú: 0 (Ó׶ùÔ°)
- ½ð±Ò: 2961
- Ìû×Ó: 425
- ÔÚÏß: 14.3Сʱ
- ³æºÅ: 247034
- ×¢²á: 2006-04-30
- רҵ: ÁÙ´²ÉúÎﻯѧ¼ìÑé
ÁÙ´²»¯Ñ§
|
¶þ¡¢ÁÙ´²»¯Ñ§ 17-ôÇƤÖÊÀà¹Ì´¼ 17-hydroxycorticosteroid, 17-OH 17-ÉúͪÀà¹Ì´¼ 17-ketogenic steroid 17-ͪÀà¹Ì´¼ 17-ketosteroid, 17-KS 2£¬3-¶þÁ×Ëá¸ÊÓÍËá 2,3-bisphosphoglycerate 3-¦Á-ôÇÀà¹Ì´¼ÍÑÇâø 3-¦Á-hydroxysteroid dehydrogenase 5¡¯-ºËÜÕËáø 5'-nucleotidase, 5'-NT CëÄ C-peptide D¸Ê¶ÌÇ D-mannose N-ÒÒõ£-¦Â-D-°±»ùÆÏÌÇÜÕø N-acetyl-¦Â-D-glucosaminidase, NAG ¦Á1¿¹Òȵ°°×ø ¦Á1-antitrypsin, AAT/¦Á1-AT ¦Á1Çòµ°°× alpha-1 globulin£¬¦Á1- globulin ¦Á1ËáÐÔÌǵ°°× ¦Á1-acid glycoprotein, AAG/¦Á1-AG ¦Á1΢Çòµ°°× ¦Á1-microglobulin, ¦Á1-MG ¦Á2¾ÞÇòµ°°× ¦Á2-macroglobulin, AMG/¦Á2-MG ¦Á2Çòµ°°× alpha-2 globulin£¬¦Á2-globulin ¦Á-L-ÑÒÔåÌÇÜÕø ¦Á-L-fucosidase, Afu ¦Â2΢Çòµ°°× ¦Â2-microglobulin, ¦Â2-MG ¦Â°ëÈéÌÇÜÕø ¦Â-galactosidase ¦ÂÄÆÄòëÄ B type natriuretic peptides, brain natriuretic peptides, BNP Óֳơ°ÄÔÄÆëÄ¡±£»¾É³Æ¡°ÄÔÄÆËØ¡± ¦ÂÇòµ°°× beta globulin£¬¦Â globulin ¦ÃÇòµ°°× gamma globulin£¬¦Ã globulin °©Åß¿¹Ô carcinoembryonic antigen, CEA °±»ù¼ºÌÇÜÕø hexosaminidase °±»ùÄ©¶Ë N-terminal Óֳơ°NÄ©¶Ë¡± °±»ùËá amino acid °±»ùËáÐòÁÐ amino acid sequence °±ÌØÒìÐԵ缫 ammonia-specific electrode °ÐÖµ target value °×£¨Ï¸°û£©ÈýÏ© leukotriene °×µ°°×/Çòµ°°×±ÈÖµ Albumin/Globulin ratio, A/G ratio °ëë×°±Ëáµ°°×øÒÖÖƼÁC cystatin C Óֳơ°ë×ÒÖËØ¡± °ëÆ×´ø¿í¶È half-band width ±ØÐèÓªÑøËØ essential nutrient ±ê׼̼ËáÇâÑÎ standard bicarbnate, SB ±í¹Û·Ö²¼ÈÝ»ý apparent volume of distribution ±ùµã½µµÍ freezing-point depression ±û°±Ëá°±»ùëÄø alanine aminopeptidase ±û°±Ëá°±»ùתÒÆø alanine aminotransferase, ALT ¾É³Æ¡°¹È±ûת°±Ã¸£¨glutamic-pyruvic transaminase,GPT£©¡± ±ûͪËá²â¶¨ pyruvic acid determination ²¡Àí»¯Ñ§ pathological chemistry ²¨³¤ wave length ±¡²ãÉ«Æ×£¨·¨£© thin-layer chromatography ²ÍºóµÄ postprandial ²Ð»ù residue ²ãÁ÷ȼÉÕÆ÷ laminar flow burner ²îʾ·Ö¹â¹â¶È²â¶¨·¨ differential spectrophotometry ²îʾÕÛÉä¼Æ differential refractometer ³¬´¿ÊÔ¼Á ultra pure reagent ³¬ÂË ultrafiltration ³¬ÉùÇåÏ´Æ÷ ultracsonic cleaner ³¬ËÙÀëÐÄ ultracentrifugation ³¬Ñõ»¯Îï᪻¯Ã¸ superoxide dismutase, SOD ³õ¼¶µ¨ÖËá primary bile acid ´¥±äÐÔ thixotropy ´«¸ÐÆ÷ transducer ´Æ¶þ´¼ estradiol, E2 ´Æ¼¤ËØ estrogen ´ÆÈý´¼ estriol, E3 ´Æͪ estrone ´Î¼¶±ê×¼ secondary standard ´Î¼¶µ¨ÖËá secondary bile acid ´Ù¼××´ÏÙ¼¤ËØ thyroid-stimulating hormone, thyrotropin TSH ´ÙÉöÉÏÏÙƤÖʼ¤ËØ adrenocorticotropic hormone, ACTH â§Ãð quenching ´ß»¯¼Á catalyst, catalyzer ´ßÈéËØ prolactin ´óÆøѹ barometric pressure£¬atmospheric pressure ´úл×ÛºÏÕ÷ metabolic syndrome µ¥°·Ñõ»¯Ã¸ monoamine oxidase, MAO µ¥±êÏßÎüÁ¿¹Ü transfer pipet µ¥ÆÏÌÑÌÇÈ©ËᵨºìËØ bilirubin monoglucuronide ¼´µ¥ÆÏÌÑÌÇÈ©Ëáõ¥ µ¥É«Æ÷ monochromator µ¥Í¨µÀ·ÖÎöÒÇ single-channel analyzer µ¨¹Ì´¼ cholesterol µ¨¹Ì´¼Ñõ»¯Ã¸ cholesterol oxidase µ¨¹Ì´¼õ¥ cholesterol ester, CE µ¨¹Ì´¼õ¥Ã¸ cholesterol esterase µ¨¹Ì´¼õ¥×ªÔ˵°°× cholesterol ester transfer protein, CETP Óֳơ°µ¨¹Ì´¼õ¥×ªÒƵ°°×¡± µ¨ºìËØ bilirubin µ¨ºìËØÑõ»¯Ã¸ bilirubin oxidase µ¨¼îõ¥Ã¸ cholinesterase, ChE µ¨Ëá cholic acid µ¨ÖËá bile acid µ°°×µçÓ¾ electrophoresis of protein µ°°×½áºÏµâ protein-bound iodine µ¼¹Ü±ê±¾£¬µ¼Äò±ê±¾ catheter specime µÈµçµã isoelectric point, pI µÈµç¾Û½¹ isoelectric focusing, IEF µÈËÙµçÓ¾ isotachophoresis µÍÃܶÈÖ¬µ°°× low density lipoprotein, LDL µÎ¶¨¹Ü buret, burette µ×Îï substrate µç£¨ÄÚ£©Éø electro-endosmosis µçÓ¾ electrophoresis µçӾͼÆ× electrphoretogram µí·Ûø amylase, AMY,AMS µí·ÛÄý½º starch gel ¶¨Öµ assigned value ¶¯Âö[Ѫ]»¯ arterialization ¶àͨµÀ·ÖÎöÒÇ multiple-channel analyzer ¶ìÍÑÑõµ¨Ëá chenodeoxycholic acid ¶ù²è·Ó°· catecholamine ¶þÑõ»¯Ì¼·Öѹ pappenheimer CO2, PCO2 ¶þÑõ»¯Ì¼º¬Á¿ carbon dioxide content ¶þÑõ»¯Ì¼½áºÏÁ¦ carbon dioxide combining power, CO2CP; CO2 combining poper, Co2CP ¶þÒÒõ£Ò»ë¿·¨ diacetyl monoxime method ·¢¹â¶þ¼«¹Ü light emitting diode ·Çµ°°×µª non-protein nitrogen, NPN ·ÇºôÎüÐÔpH nonrespiratory pH ·Ç½áºÏµ¨ºìËØ unconnect bilirubin ·Çõ¥»¯Ö¬·¾Ëá non-esterified fatty acid, free fatty acid Óֳơ°ÓÎÀëÖ¬·¾Ëᡱ¡£ ·Ö¹â¹â¶È¼Æ spectrophotometer ·ÖÁ¢Ê½·ÖÎöÒÇ discrete analyzer ·ÖÅäÆ÷ dispenser ·ÖÎöÊÔ¼Á analytical reagent ·Ö×Óɸ molecular sieve ·åŨ¶È peak concentration ·ú»¯ÄÆ sodium fluoride ¸£ÁÖ-ÎâÊÏ·¨ Folin-Wu method ¸¹Ë® ascitic fluid, ascites ¸Æ calcium ¸É»¯Ñ§ dry chemistry, solid phase chemistry Óֳơ°¹ÌÏ໯ѧ¡±¡£ ¸ÉÉæÂ˲¨Æ¬ interference filter ¸ÊÓͼ¤Ã¸ glycerol kinase ¸ÊÓÍÁ×Ëáø glycerophosphatase ¸ÊÓÍÁ×ËáÍÑÇâËá glycerol phosphate dehydrogenase ¸ÊÓÍÈýõ¥£¬Èýõ£¸ÊÓÍ triglyceride, TG ¸ÎËغóÖ¬µ°°×Ö¬·¾Ã¸ post-heparin lipoprotein lipase ¸ÎËØ»¯Ñª½¬ heparinized plasma ¸Î֬ø hepatic endothelail lipase, HL; HTGL éÏéÓÍ olive oil ¸ßÃܶÈÖ¬µ°°× high density lipoprotein, HDL ¸ßЧҺÏàÉ«Æ×£¨·¨£© high performance liquid chromatography غ[Íè]ËØ testosterone ¹¤Òµ¼¶ technical grade ¹È°±õ£×ªëÄø ¦Ã-glutamyl transpeptidase, ¦Ã-glutamyltransferase, ¦Ã-GT; GGT Óֳơ°¹È°±õ£»ùתÒÆø¡± ¹ÈŨ¶È trough concentration ¹ÌÏàø immobilized enzyme ¹âµç±¶Ôö¹Ü photomultiplier tube ¹â¶È²â¶¨·¨ photometry ¹âÃÜ¶È¼Æ densitometer ¹âÆ×´ø¿í¶È spectral band width ¹âÆ×¼¶ spectroscopic grade ¹âÉ¢Éä light scattering ¹è»¯ siliconization ¹ûÌÇ°· fructosamine ¹ûÌÇÄò fructosuria ¹ýÑõ»¯Çâø£¬´¥Ã¸ catalase ¹ýÑõ»¯Îïø peroxidase º£ÔåÌÇø trehalase ºóÒ¶¼ÓѹËØ£¬¼ÓѹËØ vasopressin, VP »¥²¹É« complementary color ¿¹ÀûÄò¼¤ËØ Antidiuretic hormone,ADH »¨ÉúËÄÏ©Ëá arachidonic acid »¬Òº synovial fluid »¯Ñ§²¡Àíѧ chemical pathology »¯Ñ§´¿ chemical pure »¯Ñ§·¢¹â chemiluminescence »·ÏÙÜÕÒ»Á×Ëá cyclic adenosine monophosphate, cAMP Óֳơ°»·ÏÙÜÕËᡱ »º³å¼î buffer base, BB »ÆÌåÉú³ÉËØ luteinizing hormone »Çäå·ÓÄÆ bromsulphalein, BSP »ð¼ýµçÓ¾ rocket electrophoresis »ðÑæ¹â¶È¼Æ flame photometer ¼¡¸Æµ°°× troponin ¼¡ôû creatinine ¼¡ôûÇå³ýÊÔÑé creatinine clearance test ¼¡Ëá creatine ¼¡Ëἤø creatine kinase, CK »ù̬ ground state »ùÏßƯÒÆ baseline shift »ùÒòоƬ gene chip, gene arrays ¼¤·¢ excitation ¼¤ËØ hormone ¼«µÍÃܶÈÖ¬µ°°× very low density lipoprotein, VLDL ¼ºÌǼ¤Ã¸·¨ hexokinase method ¼××´ÏÙÇòµ°°× thyroglobulin, Tg ¼××´ÏÙËØ thyroxine, T4 ¼××´ÏÙËؽáºÏÇòµ°°× thyroxine-binding globulin, TBG ¼Ø kalium, potassium ¼î²»×ã base deficit, BD ¼î¹ýÊ£ base excess, BE ¼îÐÔÁ×Ëáø alkaline phosphatase, ALP£¬AKP ¼îÖü alkaline reserve ½µ¸ÆËØ calcitonin ½»ÁªÆϾÛÌÇ cross-linked dextran ½Á°èÆ÷ stirrer ½áºÏµ¨ºìËØ conjugated bilirubin ½áºÏµ¨ÖËá conjugated bile acid ¾Æ¤µç¼« perculaneous electrode ¾Û±ûÏ©õ£°·Äý½º polyacrylamide gel ¿ÊÏ£¨¶¨µª£©·¨ Kjeldahl's method ¿µÎ¤À©É¢·¨ Conway diffusion method ²â°±»ò¶þÑõ»¯Ì¼µÄ΢Á¿»¯Ñ§·¨ ¿¹»µÑªËáÑõ»¯Ã¸ ascorbic acid oxidase ¿¹ÀûÄò¼¤ËØ antidiuretic hormone, ADH ¿¹Äý¼Á anticoagulant ¿¼Âí˹ÁÁÀ¶ Coomassie brilliant blue ¿Õ¸¹±ê±¾ fasting specimen ¿Ú·þÆÏÌÑÌÇÄÍÁ¿ÊÔÑé oral glucose tolerance test, OGTT À±¸ù¹ýÑõ»¯Îïø horseradish peroxidase, HRP ÀëÐÄ»ú centrifuge ÀëÐÄʽ·ÖÎöÒÇ centrifugal analyzer Àë×Ó½»»»É«Æ×£¨·¨£© ion-exchange chromatography Àë×ÓÇ¿¶È ionic strength Àë×ÓÑ¡Ôñ£¨Ä¤£©µç¼« ion-selective (membrane) electrode Àö´ººì ponceau Á¬±½Èý·Óºì pyrogallol red Á¬ÐøÁ÷¶¯Ê½·ÖÎöÒÇ continuous flow analyzer Á½ÐÔµç½âÖÊÔØÌå ampholyte carrier ÁÁ°±Ëá°±»ùëÄø leucine aminopeptidase, LAP ÁÑ϶ slit Óֳơ°ÏÁ·ì¡±¡£ ÁÚ¼×±½°··¨ o-toloidine method, ortho-toluidine method ÁÙ´²»¯Ñ§ clinical chemistry ÁÙ´²ÉúÎﻯѧ clinical biochemistry Á× phosphorus Á×¹â phosphorescence Á×Ö¬ phospholipid Á×֬ø phospholipase Á㼶·´Ó¦ zero-order reaction Á÷¶¯³Ø flow cell Óֳơ°Á÷¶¯±¡± Á÷¶¯×¢Éä·ÖÎöÒÇ flow injection analyzer Á÷ʽϸ°ûÊõ flow cytometry Â˹âƬ¹â¶È¼Æ filter photometer ÂÈ£¬ÂÈ»¯Îï chlorine, chloride ÂÑÁ×Ö¬ lecithin ÂÑÁ×Ö¬µ¨¹Ì´¼õ£»ùתÒÆø lecithin cholesterol acyltransferase, LCAT ÂÑÅݴ̼¤ËØ follicle stimulating hormone, FSH ëϸ¹ÜpHµç¼« capillary pH electrode ø enzyme øµç¼« enzyme electrode ø·¨·ÖÎö enzymatic analysis ÃŶ¬°±Ëá°±»ùתÒÆø aspartate aminotransferase, AST ¾É³Æ¡°¹È²Ýת°±Ã¸£¨glutamic-oxaloacetic transaminase,GOT£©¡± Ã×Êϳ£Êý Michaelis constant Óֳơ°Ã×Çжû³£Êý¡± Ä£¿éʽ×Ô¶¯»¯ÏµÍ³ modular automation system ĤÂËÆ÷ membrance filter Ħ¶û[Ïû¹â]ϵÊý molar absorption coefficient Ħ¶û·ÖÊý mole fraction ÄÚÉú¼¡ôûÇå³ýÂÊ endogenous creatinine clearance ÄÆ natrium, sodium ÄÎÊÏÊÔ¼Á Nessler reagent ÄÔ¼¹Òº cerebrospinal fluid, CSF ÄòÄÒËØ allantoin ÄòËصª urea nitrogen ÄòËØø·¨ urease method ÄòËá uric acid, UA ÄòËáø uricase Äý½º gel Äý½º¹ýÂË gel filtration îÏïèÂ˲¨Æ÷ didymium filter ÅÁ˹¿¨ pascal, Pa ¹ú¼ÊѹÁ¦±ê×¼µ¥Î» ƤÖÊ´¼ cortisol Ư¸¡¦ÂÖ¬µ°°× floating ¦Â-lipoprotein ÆÏÌÇÈ©Ëá»ùתÒÆø glucuronyl transferase ÆÏÌÇÈ©Ëáø glucuronidase ÆÏÌÑÌÇ-6-Á×ËáÍÑÇâø glucose-6-phosphate dehydrogenase, G-6-PD; G6PD ÆÏÌÑÌÇÄÍÁ¿ÊÔÑé glucose tolerance test ÆÏÌÑÌÇÑõ»¯Ã¸·¨ glucose oxidase method ÆøÌå²âÁ¿·¨ gasometry ÆøÏàÉ«Æ×-ÖÊÆ×ÁªÓà gas chromatography-mass spectrometry Æø-ҺɫÆ×£¨·¨£© gas-liquid chromatography Óֳơ°Æø-ÒºÏàÉ«Æס±¡£ ǨÒÆÂÊ mobility Óֳơ°Ìʶȡ±¡£ Ç°¦ÂÖ¬µ°°× pre ¦Â-lipoprotein Ç°Áл·ËØ prostacyclin Ç°ÁÐÏÙËØ Prostaglandin,PG Ç°Çåµ°°× prealbumin, PA ¾É³Æ¡°Ç°°×µ°°×¡± Ç׺ÍÉ«Æ×£¨·¨£© affinity chromatography Çåµ°°× albumin ¾É³Æ¡°°×µ°°×¡± ÇíÖ¬Äý½º agar gel ÇíÖ¬ÌÇÄý½º agarose gel Çòµ°°× globulin Çø´øµçÓ¾ zone electrophoresis È¥¼×ÉöÉÏÏÙËØ noradrenalin, norepinephrin È«Ï¢¹âÕ¤ holographic grating È©¹Ìͪ aldosterone ȾÁϽáºÏ·¨ dye-combining method ÈËÈÞëĤ´ÙÐÔÏÙ¼¤ËØ human chorionic gonadotropin, hCG ÈÝ»ý·ÖÊý volume fraction ÈÝ»ý¿Ë·Ö×ÓŨ¶È molarity Èܽâ¶È£¨¿ÉÈÜÐÔ£© solubility È䶯±Ã peristaltic pump ÈéÃÓ΢Á£ chylomicron, CM ÈéËá²â¶¨ lactic acid determination ÈéËáÍÑÇâø lactiate dehydrogenase, LD; LDH ÈéÌÇÄò lactosuria ÈûÂüЧӦ Zeeman effect Èýµâ¼×[×´]ÏÙÔ°±Ëá triiodothyronine,T3 ÈýÓÍËá¸ÊÓÍõ¥ triolein É¢Éä±È×Ç·¨ nephelometry ɨÃè¹âÃÜ¶È¼Æ scanning densitometer Óֳơ°ÃܶÈɨÃèÒÇ¡±¡£ É«°±Ëá³ÊÉ«ÊÔÑé Hopkins-Cole test Óֳơ°»ôÆÕ½ð˹-¿Æ¶ûÊÔÑ顱 É«Æ×£¨·¨£©£¬²ãÎö£¨·¨£© chromatography É«Æ×¼¶ chromatographic grade Éñ¾ÔÌØÒìÏ©´¼»¯Ã¸ neuron-specific enolase, NSE ÉöÉÏÏÙƤÖʼ¤ËØ adrenocortical hormone ÉöÉÏÏÙËØ adrenalin, epinephrin |
2Â¥2006-05-09 19:19:35
