fingerprint$28361$ - ترجمة إلى اليونانية
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fingerprint$28361$ - ترجمة إلى اليونانية

ANALYTICAL TECHNIQUE FOR PROTEIN IDENTIFICATION
Fingerprint (protein)
  • A typical workflow of a peptide mass fingerprinting experiment.

fingerprint      
n. δακτυλικό αποτύπωμα
time clock         
  • A wall-mounted time clock with biometric (fingerprint) recognition
  • Bundy clock
  • Another typical modern E-time clock
TIMEPIECE USED TO ASSIST IN TRACKING THE HOURS WORKED BY AN EMPLOYEE OF A COMPANY
Timeclock; Punch clock; Bundy clock; Clock card; Biometric time clock; Fingerprint clock; Punching a clock; Punchclock; Clock number; Time recorder; Clock card machine; Bundy Clock; Clocking machine; Clocking-in machine
ωρολόγιο που σημειώνει τις ώρες εισόδου και εξόδου κάθε εργάτου

تعريف

minutiae
The minutiae of something such as someone's job or life are the very small details of it. (FORMAL)
Much of his early work is concerned with the minutiae of rural life.
N-PLURAL: usu the N of n

ويكيبيديا

Peptide mass fingerprinting

Peptide mass fingerprinting (PMF) (also known as protein fingerprinting) is an analytical technique for protein identification in which the unknown protein of interest is first cleaved into smaller peptides, whose absolute masses can be accurately measured with a mass spectrometer such as MALDI-TOF or ESI-TOF. The method was developed in 1993 by several groups independently. The peptide masses are compared to either a database containing known protein sequences or even the genome. This is achieved by using computer programs that translate the known genome of the organism into proteins, then theoretically cut the proteins into peptides, and calculate the absolute masses of the peptides from each protein. They then compare the masses of the peptides of the unknown protein to the theoretical peptide masses of each protein encoded in the genome. The results are statistically analyzed to find the best match.

The advantage of this method is that only the masses of the peptides have to be known. Time-consuming de novo peptide sequencing is then unnecessary. A disadvantage is that the protein sequence has to be present in the database of interest. Additionally most PMF algorithms assume that the peptides come from a single protein. The presence of a mixture can significantly complicate the analysis and potentially compromise the results. Typical for the PMF based protein identification is the requirement for an isolated protein. Mixtures exceeding a number of 2-3 proteins typically require the additional use of MS/MS based protein identification to achieve sufficient specificity of identification (6). Therefore, the typical PMF samples are isolated proteins from two-dimensional gel electrophoresis (2D gels) or isolated SDS-PAGE bands. Additional analyses by MS/MS can either be direct, e.g., MALDI-TOF/TOF analysis or downstream nanoLC-ESI-MS/MS analysis of gel spot eluates.