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An ABC transporter with a secondary-active multidrug translocator domain

Author

Listed:
  • Henrietta Venter

    (University of Cambridge)

  • Richard A. Shilling

    (University of Cambridge)

  • Saroj Velamakanni

    (University of Cambridge)

  • Lekshmy Balakrishnan

    (University of Cambridge)

  • Hendrik W. van Veen

    (University of Cambridge)

Abstract

Multidrug resistance, by which cells become resistant to multiple unrelated pharmaceuticals, is due to the extrusion of drugs from the cell's interior by active transporters such as the human multidrug resistance P-glycoprotein1. Two major classes of transporters mediate this extrusion2,3. Primary-active transporters are dependent on ATP hydrolysis, whereas secondary-active transporters are driven by electrochemical ion gradients that exist across the plasma membrane. The ATP-binding cassette (ABC) transporter LmrA4 is a primary drug transporter in Lactococcus lactis that can functionally substitute for P-glycoprotein in lung fibroblast cells5. Here we have engineered a truncated LmrA protein that lacks the ATP-binding domain. Surprisingly, this truncated protein mediates a proton–ethidium symport reaction without the requirement for ATP. In other words, it functions as a secondary-active multidrug uptake system. These findings suggest that the evolutionary precursor of LmrA was a secondary-active substrate translocator that acquired an ATP-binding domain to enable primary-active multidrug efflux in L. lactis.

Suggested Citation

  • Henrietta Venter & Richard A. Shilling & Saroj Velamakanni & Lekshmy Balakrishnan & Hendrik W. van Veen, 2003. "An ABC transporter with a secondary-active multidrug translocator domain," Nature, Nature, vol. 426(6968), pages 866-870, December.
  • Handle: RePEc:nat:nature:v:426:y:2003:i:6968:d:10.1038_nature02173
    DOI: 10.1038/nature02173
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