Cepheid Flashcards
describe the general principles of qPCR
generation of products from template is detected in real time through an increase in fluorescence generated by fluorophore labels
fluorescent signal intensity > set threshold
cycle number at which fluorescent signal crosses threshold known as Ct or Cp
T or F. The Ct value is inversely proportional to the amount of starting material (template NA)
T
qPCR amplification curve
a baseline that gradually transitions into (2) an exponential region, followed by (3) a plateau, which indicates that amplification is reducing
generated based on the quantitative relationship between the fluorescence signal accumulation and cycles
explain the principles of Taqman probes aka 5’ nuclease probes
- have 5’ fluorophore and 3’ quencher
- probe intact = FRET occurs = no light detected
- DNA polymerase cleaves probe = separating fluorophore from quencher
- free fluorophore signal detected
overview of 5’ nuclease assays
- primers and probe hybdridize; sequence- dependent to complementary DNA strand; quencher absorbs fluorescence by fluorophore
- polymerase extends from primers and begins DNA synthesis
- polymerase reaches probe; exonuclease activity of pol cleaves HYBRIDIZED probe; fluorophore = signal
- fluorescence measured by real-time instrument
repeated for each PCR cycle; if intercalating dyes used = primer-dimers and non-specific producTs will contribute to fluorescence BUT Taqman is specific and fluorescence will only be produced for DNA sequence probe and primers hybridize to
explain principles of molecular beacon probes
single stranded molecule with a quencher and fluorophore at the ends
5’ end and 3’ end complementary = form hairpin so fluorophore and quencher are in close proximity and FRET occurs
when probe hybridizes to template, fluorophore and quencher separated = SIGNAL
NOTE: probe not destroyed by Taq
steps of molecular beacon probes PCR
- molecular beacon probes hybridize to target sequences = separates the Q and F (straighten from hairpin loop) = FLUORESCENCE
probes that do not hybridize, reform hairpin = no fluorescence = not detected - polymerase extend from primers and begins DNA synthesis
- polymerases displaces probe without being degraded; molecular beacons can participate in multiple rounds of annealing
- pol continues extension of primers to complete synthesis of DNA strand
explain scorpion probes (primers)
- bi-functional molecules in which a primer is covalently linked to the probe
- fluorophore and quencher
- absence of target = quencher absorbs fluorescence
- presence of target = fluorophore and quencher separate = increase in fluorescence
- fluorescence detected and measured in reaction tube
- between primer and probe is a blocker region which prevents elongation of the reverse strand
two different methods of nucleic acid extraction used i the Cepheid cartridge
physical = sonication
chemical = lysis reagent
briefly describe how the sample moves thorugh the Cepheid cartridge chambers
syringe motor raises and lowers through cartridge chambers
this action creates vacuum = pulls fluid through microvalves = moves sample and dissolved reagents from one chamber to the next
identify the physical state of Cepheid amplification PCR reagents
- PCR reagents = solid beads
- DNA polymerase, buffer, cofactors, nucleotides = enzyme beads
- primers and probes = TSR (target specific reagents) beads
- some chambers contain liquid
describe the function of SPC in Cepheid cartridge
- SPC = sample processing control: exogenous nucleic acid preloaded in cartridge that co-xtracts and co-amplifies along with the sample nucleic acids; positive control, internal control
internal control
detects PCR inhibition
four controls in Cepheid cartridge
SPC = sample processing control
PCC = probe check control (aka reagent control)
SVC = sample volume CONTROL
SAC = sample adequacy control (not in all assays)
NOTE: positive and negative external controls should be run regularly
QC batch each batch of cartridges; once per day the test is performed
PCC
probe check control aka reagent control
- fluorescence reading in the rxn tube are compared to the default settings several times during procedure before PCR stage
done to ensure the fluorophores are properly emitting and haven’t spoiled in cartridge
