| ²é¿´: 248 | »Ø¸´: 5 | ||
| ¡¾½±Àø¡¿ ±¾Ìû±»ÆÀ¼Û1´Î£¬×÷Õß³è¶ùÔö¼Ó½ð±Ò 0.5 ¸ö | ||
| µ±Ç°Ö÷ÌâÒѾ´æµµ¡£ | ||
[×ÊÔ´]
É«Æ×ÊõÓï´óÈ«
|
||
|
Àë×Ó½»»»É«Æ×·¨ ion exchange chromatography£¬IECÀë×ÓÉ«Æ×·¨ ion chromatographyÀë×ÓÒÖÖÆÉ«Æ×·¨ ion suppression chromatographyÀë×Ó¶ÔÉ«Æ×·¨ ion pair chromatographyÊèË®×÷ÓÃÉ«Æ×·¨ hydrophobic interactionchromatographyÖƱ¸ÒºÏàÉ«Æ×·¨ preparative liquid chromatographyƽÃæÉ«Æ×·¨ planar chromatographyֽɫÆ×·¨ paper chromatography±¡²ãÉ«Æ×·¨ thin layer chromatography£¬TLC¸ßЧ±¡²ãÉ«Æ×·¨ high performance thin layerchromatography£¬HPTLC½þ×Õ±¡²ãÉ«Æ×·¨ impregnated thin layerchromatographyÄý½º±¡²ãÉ«Æ×·¨ gel thin layer chromatographyÀë×Ó½»»»±¡²ãÉ«Æ×·¨ ion exchange thin layerchromatographyÖƱ¸±¡²ãÉ«Æ×·¨ preparative thin layerchromatography±¡²ã°ôÉ«Æ×·¨ thin layer rod chromatographyÒºÏàÉ«Æ×ÒÇ liquid chromatographÖƱ¸ÒºÏàÉ«Æ×ÒÇ preparative liquid chromatographÄý½ºÉø͸ɫÆ×ÒÇ gel permeation chromatographÍ¿²¼Æ÷ spreaderµãÑùÆ÷ sample applicatorÉ«Æ×Öù chromatographic column°ô×´É«Æ×Öù monolith column monolith column΢Á£Öù microparticle columnÌî³äëϸ¹ÜÖù packed capillary column¿ÕÐÄÖù open tubular column΢¾¶Öù microbore column»ìºÏÖù mixed column×éºÏÖù coupled columnÔ¤Öù precolumn±£»¤Öù guard columnÔ¤±¥ºÍÖù presaturation columnŨËõÖù concentrating columnÒÖÖÆÖù suppression column±¡²ã°å thin layer plateŨËõÇø±¡²ã°å concentrating thin layer plateÓ«¹â±¡²ã°å fluorescence thin layer plate·´Ïౡ²ã°å reversed phase thin layer plateÌݶȱ¡²ã°å gradient thin layer plateÉÕ½á°å sintered plate É«Æ×ͼ chromatogram É«Æ×·å chromatographic peak·åµ× peak base·å¸ß h£¬peak height·å¿í W£¬peak width°ë¸ß·å¿í Wh/2£¬peak width at half height·åÃæ»ý A£¬peak areaÍÏβ·å tailing areaÇ°Éì·å leading area¼Ù·å ghost peak»û·å distorted peak·´·å negative peak¹Õµã inflection pointÔµã origin°ßµã spotÇø´ø zone¸´°à multiple spotÇø´øÍÑβ zone tailing»ùÏß base line»ùÏßƯÒÆ baseline drift»ùÏßÔëÉù N£¬baseline noiseͳ¼Æ¾Ø momentÒ»½×Ôµã¾Ø ¦Ã1£¬first origin moment¶þ½×ÖÐÐÄ¾Ø ¦Ì2£¬second central momentÈý½×ÖÐÐÄ¾Ø ¦Ì3£¬third central momentÒºÏàÉ«Æ×·¨ liquid chromatography£¬LCҺҺɫÆ×·¨ liquid liquid chromatography£¬LLCÒº¹ÌÉ«Æ×·¨ liquid solid chromatography£¬LSCÕýÏàÒºÏàÉ«Æ×·¨ normal phase liquidchromatography·´ÏàÒºÏàÉ«Æ×·¨ reversed phase liquidchromatography£¬RPLCÖùÒºÏàÉ«Æ×·¨ liquid column chromatography¸ßЧҺÏàÉ«Æ×·¨ high performance liquidchromatography£¬HPLC³ß´çÅųýÉ«Æ×·¨ size exclusion chromatography£¬SECÄý½º¹ýÂËÉ«Æ×·¨ gel filtration chromatographyÄý½ºÉø͸ɫÆ×·¨ gel permeation chromatography£¬GPCÇ׺ÍÉ«Æ×·¨ affinity chromatography Õ¹¿ªÊÒ development chamber Íù¸´±Ã reciprocating pump×¢Éä±Ã syringe pumpÆø¶¯±Ã pneumatic pumpÈ䶯±Ã peristaltic pump¼ì²âÆ÷ detector΢·Ö¼ì²âÆ÷ differential detector»ý·Ö¼ì²âÆ÷ integral detector×ÜÌåÐÔÄܼì²âÆ÷ bulk property detectorÈÜÖÊÐÔÄܼì²âÆ÷ solute property detector(ʾ²î)ÕÛ¹âÂʼì²âÆ÷ [differential] refractive indexdetectorÓ«¹â¼ì²âÆ÷ fluorescence detector×ÏÍâ¿É¼û¹â¼ì²âÆ÷ ultraviolet visible detectorµç»¯Ñ§¼ì²âÆ÷ electrochemical detectorÕô·¢(¼¤¹â)¹âÉ¢Éä¼ì²âÆ÷ [laser] light scatteringdetector¹âÃÜ¶È¼Æ densitometer±¡²ãɨÃèÒÇ thin layer scannerÖùºó·´Ó¦Æ÷ post-column reactorÌå»ý±ê¼ÇÆ÷ volume marker¼Ç¼Æ÷ recorder»ý·ÖÒÇ integratorÁó·ÖÊÕ¼¯Æ÷ fraction collector¹¤×÷Õ¾ work station¹Ì¶¨Ïà stationary phase¹Ì¶¨Òº stationary liquidÔØÌå supportÖùÌî³ä¼Á column packing»¯Ñ§¼üºÏÏàÌî³ä¼Á chemically bonded phasepacking±¡¿ÇÐÍÌî³ä¼Á pellicular packing¶à¿×ÐÍÌî³ä¼Á porous packingÎü¸½¼Á adsorbentÀë×Ó½»»»¼Á ion exchanger»ùÌå matrixÔØ°å support plateÕ³ºÏ¼Á binderÁ÷¶¯Ïà mobile phaseÏ´ÍÑ(ÁÜÏ´)¼Á eluant£¬eluentÕ¹¿ª¼Á developerµÈË®ÈݼÁ isohydric solvent¸ÄÐÔ¼Á modifierÏÔÉ«¼Á color [developing] agent ËÀʱ¼ä t0£¬dead time±£Áôʱ¼ä tR£¬retention timeµ÷Õû±£Áôʱ¼ä t'R£¬adjusted retention timeËÀÌå»ý V0£¬dead volume±£ÁôÌå»ý vR£¬retention volumeµ÷Õû±£ÁôÌå»ý v'R£¬adjusted retention volumeÖùÍâÌå»ý Vext£¬extra-column voluneÁ£¼äÌå»ý V0£¬interstitial volume(¶à¿×Ìî³ä¼ÁµÄ)¿×Ìå»ý VP£¬pore volume of porouspackingÒºÏà×ÜÌå»ý Vtol£¬total liquid volumeÏ´ÍÑÌå»ý ve£¬elution volumeÁ÷ÌåÁ¦Ñ§Ìå»ý vh£¬hydrodynamic volumeÏà¶Ô±£ÁôÖµ ri.s£¬relative retention value·ÖÀëÒò×Ó ¦Á£¬separation factorÁ÷¶¯ÏàǨÒƾàÀë dm£¬mobile phase migrationdistanceÁ÷¶¯ÏàÇ°ÑØ mobile phase frontÈÜÖÊǨÒƾàÀë ds£¬solute migration distance±ÈÒÆÖµ Rf£¬Rf value¸ß±ÈÒÆÖµ hRf£¬high Rf valueÏà¶Ô±ÈÒÆÖµ Ri.s£¬relative Rf value±£Áô³£ÊýÖµ Rm£¬Rm value°åЧÄÜ plate efficiencyÕۺϰå¸ß hr£¬reduced plate height·ÖÀë¶È R£¬resolutionÒºÏàÔغÉÁ¿ liquid phase loadingÀë×Ó½»»»ÈÝÁ¿ ion exchange capacity¸ºÔØÈÝÁ¿ loading capacityÉø͸¼«ÏÞ permeability limitÅųý¼«ÏÞ Vh£¬max£¬exclusion limitÍÏβÒò×Ó T£¬tailing factorÖùÍâЧӦ extra-column effect¹Ü±ÚЧӦ wall effect¼ä¸ô±ÛЧӦ spacer arm effect±ßԵЧӦ edge effect°ßµã¶¨Î»·¨ localization of spot·ÅÉä×ÔÏÔÓ°·¨ autoradiographyÔ붨Á¿ in situ quantitationÉúÎï×ÔÏÔÓ°·¨ bioautography¹éÒ»·¨ normalization methodÄڱ귨 internal standard methodÍâ±ê·¨ external standard methodµþ¼Ó·¨ addition method ÆÕÊÊУ׼(ÇúÏß¡¢º¯Êý) calibration function or curveÆ×´øÀ©Õ¹(¼Ó¿í) band broadening(·ÖÀë×÷ÓõÄ)У׼º¯Êý»òУ׼ÇúÏß universalcalibration function or curve [of separation]¼Ó¿íУÕý broadening correction¼Ó¿íУÕýÒò×Ó broadening correction factorÈܼÁÇ¿¶È²ÎÊý ¦Å0£¬solvent strength parameterÏ´ÍÑÐòÁÐ eluotropic seriesÏ´ÍÑ(ÁÜÏ´) elutionµÈ¶ÈÏ´ÍÑ gradient elutionÌݶÈÏ´ÍÑ gradient elution(ÔÙ)Ñ»·Ï´ÍÑ recycling elutionÏßÐÔÈܼÁÇ¿¶ÈÏ´ÍÑ linear solvent strength gradient³ÌÐòÈܼÁ programmed solvent³ÌÐòѹÁ¦ programmed pressure³ÌÐòÁ÷ËÙ programmed flowÕ¹¿ª developmentÉÏÐÐÕ¹¿ª ascending developmentÏÂÐÐÕ¹¿ª descending developmentË«ÏòÕ¹¿ª two dimensional development»·ÐÎÕ¹¿ª circular developmentÀëÐÄÕ¹¿ª centrifugal developmentÏòÐÄÕ¹¿ª centripetal development¾¶ÏòÕ¹¿ª radial development¶à´ÎÕ¹¿ª multiple development·Ö²½Õ¹¿ª stepwise developmentÁ¬ÐøÕ¹¿ª continuous developmentÌݶÈÕ¹¿ª gradient developmentÔȽ¬Ìî³ä slurry packingÍ£Á÷½øÑù stop-flow injection·§½øÑù valve injectionÖùÉϸ»¼¯ on-column enrichmentÁ÷³öÒº eluateÖùÉϼì²â on-column detectionÖùÊÙÃü column lifeÖùÁ÷ʧ column bleedingÏÔÆ× visualization»î»¯ activation·´³å back flushingÍÑÆø degassing¹µÁ÷ channeling¹ýÔØ overloading ÖÐÎÄ Ó¢ÎÄ É«Æ×ͼ chromatogram É«Æ×·å chromatographic peak ·åµ× peak base ·å¸ß h£¬peak height ·å¿í W£¬peak width °ë¸ß·å¿í Wh/2£¬peak width at half height ·åÃæ»ý A£¬peak area ÍÏβ·å tailing area Ç°Éì·å leading area ¼Ù·å ghost peak »û·å distorted peak ·´·å negative peak ¹Õµã inflection point Ôµã origin °ßµã spot Çø´ø zone ¸´°à multiple spot Çø´øÍÑβ zone tailing »ùÏß base line »ùÏßƯÒÆ baseline drift »ùÏßÔëÉù N£¬baseline noise ͳ¼Æ¾Ø moment Ò»½×Ôµã¾Ø ¦Ã1£¬first origin moment ¶þ½×ÖÐÐÄ¾Ø ¦Ì2£¬second central moment Èý½×ÖÐÐÄ¾Ø ¦Ì3£¬third central moment ÒºÏàÉ«Æ×·¨ liquid chromatography£¬LC ҺҺɫÆ×·¨ liquid liquid chromatography£¬LLC Òº¹ÌÉ«Æ×·¨ liquid solid chromatography£¬LSC ÕýÏàÒºÏàÉ«Æ×·¨ normal phase liquid chromatography ·´ÏàÒºÏàÉ«Æ×·¨ reversed phase liquid chromatography£¬RPLC ÖùÒºÏàÉ«Æ×·¨ liquid column chromatography ¸ßЧҺÏàÉ«Æ×·¨ high performance liquid chromatography£¬HPLC ³ß´çÅųýÉ«Æ×·¨ size exclusion chromatography£¬SEC Äý½º¹ýÂËÉ«Æ×·¨ gel filtration chromatography Äý½ºÉø͸ɫÆ×·¨ gel permeation chromatography£¬GPC |
»Ø¸´´ËÂ¥» ²ÂÄãϲ»¶
Ò»Ö¾Ô¸0703»¯Ñ§ÕÐ61×îÖÕÅÅÃû62»¯Ñ§Çóµ÷¼Á
ÒѾÓÐ32È˻ظ´
-
»¯¹¤Ñ§Ë¶294·Ö£¬Çóµ¼Ê¦ÊÕÁô
ÒѾÓÐ16È˻ظ´
-
¿¼ÑÐÓ¢Ò»ÊýÒ»338·Ö
ÒѾÓÐ7È˻ظ´
-
302Çóµ÷¼Á
ÒѾÓÐ6È˻ظ´
-
271Çóµ÷¼Á
ÒѾÓÐ25È˻ظ´
-
266µ÷¼Á
ÒѾÓÐ10È˻ظ´
-
ÉúÎïѧµ÷¼Á
ÒѾÓÐ11È˻ظ´
-
Çóµ÷¼Á
ÒѾÓÐ8È˻ظ´
-
085801µçÆøר˶272Çóµ÷¼Á
ÒѾÓÐ10È˻ظ´
-
Ò»Ö¾Ô¸ÄÏ¿Æ´óÉúÎïѧ297·Ö£¬Çóµ÷¼ÁÍƼö
ÒѾÓÐ11È˻ظ´
2Â¥2006-11-24 21:12:45
4Â¥2007-03-08 15:36:26
5Â¥2007-03-27 13:40:26
Ö§³Öһϣ¡£¡£¡ 6Â¥2007-03-28 20:37:34
¼òµ¥»Ø¸´
zhangjs3Â¥
2006-11-24 23:13
»Ø¸´
Ö§³Ö£¬£¬£¬
