<p>Many advantages come from working with β-lactamase. It shows high catalytic efficiency and simple kinetics. Also, no orthologs of <i>amp</i>R are known to be encoded by eukaryotic cells and no toxicity was identified making this protein very useful in studies involved eukaryotes (Qureshi, 2007). β-lactamase has been used to track pathogens in infected murine models (Kong <i>et al.</i>, 2010). However, in addition to its application in eukaryotic cells, β-lactamase efficiently cleaves a wide variety of substrates but its versatility goes beyond that; <i>amp</i>R preserves its activity even when fused to heterologous protein (Moore <i>et al.</i>, 1997). This feature, in particular, makes β-lactamase a potentially valuable tool for assembly of synthetic constructs.</p>
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<p>Many advantages come from working with β-lactamase. It shows high catalytic efficiency and simple kinetics. Also, no orthologs of <i>amp</i>R are known to be encoded by eukaryotic cells and no toxicity was identified making this protein very useful in studies involved eukaryotes (Qureshi, 2007). β-lactamase has been used to track pathogens in infected murine models (Kong <i>et al.</i>, 2010). However, in addition to its application in eukaryotic cells, <i>amp</i>R has been found to have an alternative application in synthetic proteins as well. <i>amp</i>R is able to preserve its activity when fused to other proteins, meaning it can viably be used in fusion proteins (Moore <i>et al.</i>, 1997). This feature, in particular, makes β-lactamase a potentially valuable tool for assembly of synthetic constructs.</p>
<h2>How is β-lactamase used as a Reporter?</h2>
<h2>How is β-lactamase used as a Reporter?</h2>
<p>β-lactamase, in the presence of different substrates, can give various outputs. It can produce a fluorogenic output in the presence of a cephalosporin derivative (CCF2/AM) and enzymatic activity can be detected by a fluorometer (Remy <i>et al</i>., 2007).</p>
<p>β-lactamase, in the presence of different substrates, can give various outputs. It can produce a fluorogenic output in the presence of a cephalosporin derivative (CCF2/AM) and enzymatic activity can be detected by a fluorometer (Remy <i>et al</i>., 2007).</p>
β-lactamase is an enzyme encoded by the ampicillin resistance gene (ampR) frequently present in plasmids for selection. Structurally, β-lactamase is a 29 kDa monomeric enzyme (Figure 1). Its enzymatic activity provides resistance to β-lactam antibiotics such as carbapenems, penicillin and ampicillin through hydrolysis of the β-lactam ring, a structure shared by the β-lactam class of antibiotics (Qureshi, 2007).
Many advantages come from working with β-lactamase. It shows high catalytic efficiency and simple kinetics. Also, no orthologs of ampR are known to be encoded by eukaryotic cells and no toxicity was identified making this protein very useful in studies involved eukaryotes (Qureshi, 2007). β-lactamase has been used to track pathogens in infected murine models (Kong et al., 2010). However, in addition to its application in eukaryotic cells, ampR has been found to have an alternative application in synthetic proteins as well. ampR is able to preserve its activity when fused to other proteins, meaning it can viably be used in fusion proteins (Moore et al., 1997). This feature, in particular, makes β-lactamase a potentially valuable tool for assembly of synthetic constructs.
How is β-lactamase used as a Reporter?
β-lactamase, in the presence of different substrates, can give various outputs. It can produce a fluorogenic output in the presence of a cephalosporin derivative (CCF2/AM) and enzymatic activity can be detected by a fluorometer (Remy et al., 2007).
Besides fluorescence assays, β-lactamase can also be used to obtain colourimetric outputs by breaking down synthetic compounds such as nitrocefin (Figure 2). The colour change goes from yellow to red (Remy et al., 2007). Colourimetric assays can also be done with benzylpenicillin as the substrate, which, gives a pH output that can be detected with pH indicators to give a colourimetric output (Li et al., 2008).