Inhibition of 2A-mediated ‘Cleavage' of Certain Artificial Polyproteins Bearing N-terminal Signal Sequences. - Archive ouverte HAL Accéder directement au contenu
Article Dans Une Revue Biotechnology Journal Année : 2009

Inhibition of 2A-mediated ‘Cleavage' of Certain Artificial Polyproteins Bearing N-terminal Signal Sequences.

Garry Alec Luke
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Jeremy Brown
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Pablo de Felipe
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Résumé

Where 2A oligopeptide sequences occur within open reading frames (ORFs), the formation of the glycyl-prolyl peptide bond at the C-terminus of (each) 2A does not occur. This property can be used to concatenate sequences encoding several proteins into a single ORF: each component of such an artificial polyprotein is generated as a discrete translation product. 2A and ‘2A-like' sequences have become widely utilised in biotechnology and biomedicine. Individual proteins may also be co- and post-translationally targeted to a variety of sub-cellular sites. In the case of polyproteins bearing N-terminal signal sequences we observed, however, that the protein downstream of 2A (no signal) was translocated into the endoplasmic reticulum (ER). We interpreted these data as a form of “slipstream” translocation: downstream proteins, without signals, were translocated through a translocon pore already formed by the signal sequence at the N-terminus of the polyprotein. Here we show this effect is, in fact, due to inhibition of the 2A reaction (formation of fusion protein) by the C-terminal region (immediately upstream of 2A) of some proteins when translocated into the ER. Solutions to this problem include the use of longer 2As (with a favourable upstream context), or, modifying the order of proteins comprising polyproteins.

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Dates et versions

hal-00540527 , version 1 (27-11-2010)

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Martin Denis Ryan, Garry Alec Luke, Jeremy Brown, Pablo de Felipe. Inhibition of 2A-mediated ‘Cleavage' of Certain Artificial Polyproteins Bearing N-terminal Signal Sequences.. Biotechnology Journal, 2009, 5 (2), pp.213. ⟨10.1002/biot.200900134⟩. ⟨hal-00540527⟩

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