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  • ¿µ¹®
    ÇѱÛ
  • delayed sleep phase
    ¼ö¸éÀ§»óÁö¿¬
  • delayed sleep phase syndrome
    ¼ö¸éÀ§»óÁö¿¬ÁõÈıº
  • depressive phase
    ¿ì¿ï»ó
  • death phase
    »ç¸ê±â
  • diastolic phase
    È®Àå±â
  • disperse phase
    ºÐ»ê±â
  • diurnal phase
    ÁÖ°£»ó
  • expiratory phase
    È£±â»ó
  • expiratory phase time
    ³¯¼û½Ã°£, È£±â½Ã°£
  • exponential phase
    Áö¼öÁõ½Ä±â
  • ejection phase
    ¹ÚÃâ±â
  • equilibrium phase
    ÆòÇü±â
  • erythrocytic phase
    ÀûÇ÷±¸³»¹ßÀ°±â
  • growth phase
    Áõ½Ä±â
  • intuitive phase
    Á÷°ü±â
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  • ¿µ¹®
    ÇѱÛ
  • phase axis
    ˤȗ̈
  • phase shift artifact
    À§»óº¯À§Àΰø¹°
  • phase wraparound artifact
    À§»óÆ÷ÀåÀΰø¹°
  • bulk phase model
    µ¢¾î¸®À§»ó¸ðÇü
  • circadian-phase intervention
    ÀÏÁÖ±âÀ§»óÁßÀç
  • colostral phase
    ùÁ¥±â, ÃÊÀ¯±â
  • compression phase
    ¾ÐÃà»ó
  • phase coherence
    À§»ó°áÁý
  • phase constant
    À§»ó»ó¼ö
  • phase curve
    À§»ó°î¼±
  • death phase
    »ç¸ê±â
  • delayed sleep phase
    Áö¿¬¼ö¸éÀ§»ó
  • delayed sleep phase syndrome
    ¼ö¸éÀ§»óÁö¿¬ÁõÈıº
  • depressive phase
    ¿ì¿ï»ó
  • diastolic phase
    È®Àå±â, À̿ϱâ
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  • ¿µ¹®
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  • inadequate luteal phase
    Ȳü±âºÎÀü(üÜô÷ÐïÝÕîï).
  • inspiratory phase
    Èí±â»ó(ýåѨßÓ).
  • inspiratory phase time
    Èí±â»ó½Ã°£.
  • phallic stage (phase)
    ³²±Ù±â(ÑûÐÆÑ¢).
  • phase
    »ó, ±â
  • phase
    ˤȗ
  • phase 1 study
    ÀÓ»óÁ¦1»ó½ÃÇè.
  • phase I block
    Á¦1»óÂ÷´Ü.
  • phase advance
    »óÀüÁø(ßÓîñòä)
  • phase angle
    À§»ó°¢(êÈßÓÊÇ).
  • phase angle
    À§»ó °¢
  • phase artifact
    À§»ó Àΰø¹°
  • phase axis
    ˤȗ ̈
  • phase boundary
    »ó°è(Ë×Ë­).
  • phase boundary force
    »ó°è(Àü)·Â(ßÓÍ£ ï³æ³).
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  • contrast sensitivity
    ´ëºñ°¨µµ
  • contrast sensitivity chart
    ´ëºñ°¨µµÇ¥
  • contrast staining
    ´ëÁ¶¿°»ö
  • contrast to noise ratio
    ´ëÁ¶ ÀâÀ½ºñ
  • double contrast arthrography
    ÀÌÁß Á¶¿µ °üÀýÁ¶¿µ¼ú
  • double contrast arthrography
    °üÀý ÀÌÁß Á¶¿µ¼ú.
  • double contrast radiography
    ÀÌÁß Á¶¿µ ¹æ»ç¼±ÃÔ¿µ¼ú
  • dynamic susceptibility contrast technique
    ¿ªµ¿ ÀÚÈ­À² ´ëÁ¶ ±â¹ý
  • gadolinium (Gd) based contrast agent
    °¡µ¹¸®´½ Á¶¿µÁ¦
  • good contrast
    ¶Ñ·ÇÇÑ ´ëÁ¶µµ
  • hepato renal echo contrast
    °£ ½ÅÀå ¿¡ÄÚ ´ëÁ¶
  • hepato-renal echo contrast
    °£-½ÅÀå (ÊÜ-ãìíô) ¿¡ÄÚ ´ëÁ¶ (ÓßðÎ), °£-½ÅÀå (ÊÜ-ãì
  • magnetic transfer contrast (MTC)
    ÀÚÈ­ Àü´Þ ´ëÁ¶µµ
  • negative contrast medium
    À½¼º Á¶¿µÁ¦
  • opaque enema =barium e., contrast e.
    ¹æ»ç Á¶¿µÁÖÀå(ðãç¯ñ¼ ).
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  • phase cancellation artifact
    À§»ó¸»¼Ò(»ó¼â)Àΰø¹°
  • phase coherence
    À§»ó°áÁý
  • phase conjugate symmetry
    À§»óȸº¹´ëĪ, À§»ó°ø¾×´ëĪ
  • phase curve
    À§»ó°î¼±
  • phase display
    À§»óÇ¥½Ã
  • phase encode direction
    À§»óºÎȣȭ¹æÇâ
  • phase encoding
    À§»óºÎȣȭ
  • phase encoding gradient
    À§»óºÎȣȭ°æ»çµµ(Àå)
  • phase encoding step
    À§»óºÎÈ£´Ü°è
  • phase evolution of fat suppression
    À§»ó¼±È¸ Áö¹æ¾ïÁ¦
  • phase frequency swap
    À§»óÁ֯ļö±³È¯
  • phase image
    À§»ó¿µ»ó
  • phase mismapping
    À§»ó¿ÀÁöµµÀÛ¼º
  • phase offset multiplannar [=POMP] imaging
    À§»ó¿ÀÇÁ¼Â´Ù¸é¿µ»ó
  • phase sensitive technique description
    À§»ó¹Î°¨¹ý¼³¸í
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DCBE double contrast barium enema
HOCM high-osmolar contrast medium; hypertrophic obstructive cardiomyopathy
LOCM low molecular contrast medium
MCE medical care evaluation; military clinical engineering; multicystic encephalopathy; multiple cartila...
MTS Medicare transaction system; magnetization transfer contrast; methotrexate; multicellular tumor sphe...
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FESEM Field Emission Scanning Electron Microscopy
FLIM Fluorescence lifetime imaging microscopy
HREM High Resolution Electron Microscopy
HVEM High Voltage Electron Microscopy
HRTEM High resolution transmission electron microscopy
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  • luteal phase
    ¿ù°æ ÁÖ±âÁß È²Ã¼±â, Ȳü ´Ü°è, Ȳü±â
  • lysogenic phase
    ¿ë¿ø±â
  • maximal ejection phase
    ÃÖ´ë ±¸Ãâ±â
  • mitotic phase
    À¯»ç ºÐ¿­±â
  • phase 1 study
    ÀÓ»ó Á¦1»ó ½ÃÇè
  • phase artifact
    À§»ó Àΰø¹°
  • phase boundary
    »ó°è
  • phase coherence
    À§»ó °áÁý
  • phase curve
    À§»ó °î¼±
  • phase display
    À§»ó Ç¥½Ã
  • phase encoding
    À§»ó ºÎȣȭ
  • phase encoding step
    À§»ó ºÎÈ£ ´Ü°è
  • phase frequency swap
    À§»ó Á֯ļö ±³È¯
  • phase II treatment
    Á¦2´Ü°è Ä¡·á
  • phase mismapping
    À§»ó ¿ÀÁöµµ ÀÛ¼º
CancerWEB ¿µ¿µ ÀÇÇлçÀü À¯»ç °Ë»ö °á°ú : 15 ÆäÀÌÁö: 4
microscopy, immunoelectron Microscopy in which the samples are first stained immunocytochemically and then examined using an electron microscope. Immunoelectron microscopy is used extensively in diagnostic virology as part of very sensitive immunoassays.
(12 Dec 1998)
microscopy, interference Microscopy in which physiological and photometric contrast in the image is influenced or produced by the action of optical components which regulate interference.
(12 Dec 1998)
microscopy, polarization Microscopy using polarised light in which phenomena due to the preferential orientation of optical properties with respect to the vibration plane of the polarised light are made visible and correlated parameters are made measurable.
(12 Dec 1998)
microscopy, scanning tunneling Electron microscopy in which a very sharp conducting needle is swept just a few angstroms above the surface of a sample. The tiny tunneling current that flows between the sample and the needle tip is measured and from this are produced three-dimensional topographs, with a lateral resolution often as good as 1-2 angstroms and a vertical resolution of less than 1 angstrom. Due to their composition, biological samples are usually coated with a conductive layer, e.g., by depositing a thin metal or carbon film on top of the sample, to enhance their conductivity.
(12 Dec 1998)
microscopy, ultraviolet Microscopy in which the image is formed by ultraviolet radiation and is displayed and recorded by means of photographic film.
(12 Dec 1998)
microscopy, video Microscopy in which television cameras are used to brighten magnified images that are otherwise too dark to be seen with the naked eye. It is used frequently in telepathology.
(12 Dec 1998)
confocal microscopy <procedure> A system of (usually) epifluorescence light microscopy in which a fine laser beam of light is scanned over the object through the objective lens. The technique is particularly good at rejecting light from outside the plane of focus and so produces higher effective resolution than is normally achieved.
(18 Nov 1997)
Conventional Transmission Electron Microscopy <technique> A term applied to 'normal' transmission electron microscopy imaging. The electron beam is passed through a thin film sample (typically ~1-200 nm thick). Bright field diffraction contrast images are formed with the direct (undiffracted) beam. Dark field images are formed with a selected diffracted beam. CTEM imaging is used in the general observation of samples and careful selection of the diffracting conditions of the sample will allow the analysis of defect structures within the sample.
(05 Aug 1998)
polarization microscopy <procedure> Any form of microscopy capable of detecting birefringent objects. Usually performed with a polarizing element below the stage to produce plane polarized light and an analyser that is set to give total extinction of the background and thus to detect any birefringence.
(18 Nov 1997)
scanning electron microscopy <procedure> Technique of electron microscopy in which the specimen is coated with heavy metal and then scanned by an electron beam. The image is built up on a monitor screen (in the same way as the raster builds a conventional television image). The resolution is not so great as with transmission electron microscopy, but preparation is easier (often by fixation followed by critical point drying), the depth of focus is relatively enormous, the surface of a specimen can be seen (though not the interior unless the specimen is cracked open) and the image is aesthetically pleasing.
(18 Nov 1997)
Scanning Probe Microscopy <technique> Initially called Atomic Force Microscopy, this technique is now more typically termed Scanning Force Microscopy or Scanning Probe Microscopy.
This instrument is essentially an extremely high resolution profilometre. A sharp tip, typically fabricated from silicon nitride, is scanned across the surface of a sample at a constant force by three piezoelectric ceramics.
The piezoelectric ceramics are computer controlled via a feedback loop which monitors the position of the tip by means of an optical lever. (A laser is focused on the top of the tip support and the beam reflected into a position sensitive detector). The changes in height of the tip are used to form an image as the tip is scanned across the sample.
Acronym: SPM
(26 Mar 1998)
scanning transmission electron microscopy <procedure> Method of electron microscopy in which image formation depends upon analysis of the pattern of energies of electrons that pass through the specimen. Has comparable resolving power to conventional transmission EM.
(18 Nov 1997)
scanning tunnelling microscopy <procedure> A form of ultra high resolution microscopy of a surface in which a very small current is passed through a surface and is detected by a microprobe of atomic dimnensions at its tip that scans the surface by use of a piezodrive. In the simplest form the current transferred to the probe is recorded as an indication of the contours of molecules on the surface above the local plane. In more complex forms feedback is used to hold the probe at a constant difference and the signal in the feedback loop indicates the contours of the molecule. Capable of resolving single atoms and known to work for nonconducting molecules as well as conducting ones.
(18 Nov 1997)
high extinction microscopy <technique> Polarized-light, interference, fluorescence, and other modes of microscopy using polarization rectifiers and other devices to achieve a high degree of back- ground extinction in order to bring out the signal originating from a very small degree of birefringence, optical path difference, fluorescence etc.
(05 Aug 1998)
holographic microscopy <technique> A mode of light microscopy in which a highly coherent, laser beam is split into a reference and main beam, with the reference beam (usually travelling outside of the microscope) being made to interfere with the main beam that has passed through the specimen. The interference of the two mutually coherent beams forms a hologram. The depth of field gained by viewing the hologram is essentially infinitely great, and the contrast mode or observation can be switched to dark field, phase contrast, interference contrast, etc., after the hologram has been formed by the microscope in bright field.
(05 Aug 1998)
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