In a collaboration initiated by Chris Ponting, we have also identified the family of proteins identified by Bruno Martoglio and colleagues (Ponting et al. 2000) [1]. In that paper we speculated that these presenilin homologs (PSH), as we called them, were likely to be proteases based on the evidence that PS were proteases. The study by Martoglio provides almost unequivocal proof that the protein they identified and named signal peptide peptidase (SPP, which we referred to as PSH3), is a protease capable of cleaving a signal peptide. This paper is simply an outstanding study that should convince many, if not all, in the field about the nature of this class of proteins. PS and PS-like proteins not only appear to be proteases but, as proposed by Wolfe and colleagues, aspartyl proteases [3]. Future studies on other PSH should also reveal that they possess proteolytic activity, and reveal even more research opportunities for those interested in studying intramembranous proteolytic cleavage events carried out by multipass membrane proteases.
In my mind, this settles the debate over the role of PS in gamma-secretase cleavage. PS are almost certainly the catalytic components of a gamma-secretase complex. To make clear my reasoning, I will review the data on PS that support their catalytic role and also answer the criticisms put forth by others. Of course PS do not appear capable of catalyzing gamma-cleavages by themselves. Two other components necessary for this cleavage are Nicastrin and a membrane environment rich in cholesterol. Other as yet unidentified factors may also be required for cleavage.
First, all of the genetic evidence is consistent with PS being gamma-secretase. FAD-linked PS mutations alter gamma-cleavage and the combined PS 1 and 2 knockout completely abolishes gamma-cleavage. We believe that reports showing otherwise are technically flawed. (However, it is possible that other minor pathways for gamma-like cleavages exist, see concluding paragraph).
Second, biochemical evidence supports this concept. PS co-purify and are enriched as one purifies gamma-secretase activity. This occurs no matter how the purification is carried out. Purifications using inhibitor affinity columns, immunoprecipitations, or just differential centrifugation or other physical separations all reveal the same thing. PS and nicastrin co-purify with gamma-secretase activity. Moreover, mutations of either of the critical aspartates in PS, deletion of the first two transmembrane domains, or the naturally occurring mutation insR352 all result in dominant-negative PS molecules. Although possible, it is hard to see how all of these alterations could alter a co-factor function in the same way.
Certainly these studies are potentially consistent with PS being a co-factor and not catalytic, but the third line of evidence is not. This evidence is pharmacologic in nature. All gamma-secretase inhibitors that have been rigorously tested appear to bind PS. Most convincingly, protease inhibitors designed to inhibit aspartyl proteases bind directly to PS. In this regard, the studies by Weihofen et al. further demonstrate the importance of the aspartates in catalysis, as mutation of the aspartate abolishes inhibitor binding. Of course, not all inhibitors of gamma-secretase that bind PS look like typical protease inhibitors, but this is not particularly relevant to the debate. Given a novel class of proteases, novel inhibitors will be identified. (If they were willing, it would be interesting to actually poll companies with active or defunct gamma-secretase programs to ask them how many of their gamma-inhibitors they have found bind to presenilin. My sense is that anyone who has looked finds this to be the case).
So what are the remaining objections?
First: PS doesn't look like typical proteases.
Well, neither does rhomboid, an intramembranous-cleaving serine protease [4], or site-two protease, an intramembranous-cleaving metalloprotease that cleaves the SREBP [5]. Should we expect these proteins to closely resemble known proteases? The remarkable fact is that the catalytic mechanism may be analogous to other classes of enzymes, and that catalytic residues do in fact appear to be conserved. Indeed, the demonstration that SPP is almost certainly a protease just makes us aware that we should be prepared to expect the unexpected.
Second: We can't reconstitute gamma-secretase activity.
This certainly is a valid criticism but represents a technical shortcoming, not a conceptual one. Gamma-secretase activity is associated with a high-molecular weight complex that appears to require Nicastrin as well [6-9], and perhaps other unidentified proteins. However membrane environment is also crucial for this cleavage (at least for AβPP cleavage) with membrane cholesterol content being a prime determinant of activity [10]. Given the nature of this complex it may very well be difficult to reconstitute activity, especially if we haven't identified all the players. Indeed, the activity of the best-known intramembranous cleaving protease, site-two protease, has yet to be reconstituted. Moreover, no one to my knowledge has purified from scratch the best-known multi-subunit protease, the proteasome. Yet there is no debate about its proteolytic activity. In this regard, I guess that it will be easier to purify the complex to homogeneity than it will be to reconstitute activity.
Third: The spatial paradox, i.e. PS are not in the right place in the cell.
This criticism has been overplayed. First, evidence in multiple systems suggests that PS and substrate co-localize and co-fractionate. Indeed, one can co-purify PS with substrate especially when gamma-inhibitors are around [9]. Moreover, studies in the brain show that substrate and PS co-localize quite well [11]. Second, it is possible that a small amount of PS can turn over a lot of substrate. If this is so, it may be hard to show co-localization of activity with substrate if a lot of inactive PS is around, too. Third, it is also possible that PS epitopes are buried when they are in the active complex, preventing one from seeing PS in places where substrate might exist. Finally, it is entirely possible that substrate is being actively trafficked to a site in the cell containing active PS/gamma-secretase. Thus, the interaction, when unperturbed, would be transient and difficult to localize.
Fourth: Activity paradoxes.
There are studies that claim PS aspartate mutations do not have dominant-negative effects on cleavage of certain substrates. In our hands D257, D385E, delTM-12 and insR352 inhibit Aβ production and Notch cleavage to nearly equivalent extents. Marked inhibition of Aβ production is also reported in the Zheng paper (see related news item) where the D257A PS is expressed in vivo. To infer that PS are unlikely to be gamma-secretase from reports showing differential inhibition of Notch and Aβ production to me seems to be a stretch. In all cases, substrate accumulates. We believe that, under certain circumstances, such substrate accumulation can overcome partial gamma-secretase inhibition that occurs when these dominant-negative PS are expressed, and we have unpublished data that supports this belief. Indeed, if substrate accumulates fivefold and the enzyme activity is reduced by 20 percent, you should get the same amount of product (assuming a simple first-order kinetic model). The difference in product that is seen likely has to deal with substrate turnover, trafficking of substrates, and levels of substrate to start.
For some time I struggled with the notion that PS were gamma-secretase because one could differentially inhibit Aβ40 and Aβ42 production [12], whereas a knockout of PS1 affects both equally and a combined PS knockout abolishes Aβ production [13-15]. Indeed, in a grant proposal in 1999, based on data from inhibitors such as pepstatin, I hypothesized that gamma-secretase activity was likely to be attributed to two closely related aspartyl proteases. I reconcile this today by hypothesizing that PS exist in multiple conformations/complexes that may carry out different cleavages and can be differentially inhibited. If gamma-secretase can exist in various conformations or complexes that have different activities, it is easy to see how mutations and inhibitors can have differential effects on cleavage at various sites or various substrates.
In conclusion, I think the vast majority of evidence points to a catalytic role for PS in gamma-secretase cleavage. Those who believe otherwise will need to find another protease in the gamma-complex and show that it is the real gamma-secretase in order to reinvigorate the debate. Despite my confidence that PS are the catalytic component of gamma-secretase, however, I think the question whether PS are the only gamma-secretase is worthy of further evaluation. There are some reports that do suggest that Notch and AβPP can under certain circumstances undergo gamma-like cleavages that do not appear to be PS-dependent. These do not appear to be major pathways for production of Aβor NICD like products, but may very well be real. Perhaps, PSH/SPP family members will prove to be responsible.
References:
1. Ponting, C.P., et al., Identification of a novel family of presenilin homologues. Hum Mol Genet, 2002. 11(9): p. 1037-44.
3. Wolfe, M.S., et al., Two transmembrane aspartates in presenilin-1 required for presenilin endoproteolysis and gamma-secretase activity. Nature, 1999. 398(6727): p. 513-517.
4. Urban, S., J.R. Lee, and M. Freeman, Drosophila rhomboid-1 defines a family of putative intramembrane serine proteases. Cell, 2001. 107(2): p. 173-82.
5. Brown, M.S., et al., Regulated intramembrane proteolysis: a control mechanism conserved from bacteria to humans. Cell, 2000. 100(4): p. 391-8.
6. Kopan, R. and A. Goate, Aph-2/Nicastrin: an essential component of gamma-secretase and regulator of Notch signaling and Presenilin localization. Neuron, 2002. 33(3): p. 321-4.
7. Yu, G., et al., Nicastrin modulates presenilin-mediated notch/glp-1 signal transduction and betaAPP processing [see comments]. Nature, 2000. 407(6800): p. 48-54.
8. Hu, Y., Y. Ye, and M.E. Fortini, Nicastrin is required for gamma-secretase cleavage of the Drosophila Notch receptor. Dev Cell, 2002. 2(1): p. 69-78.
9. Esler, W.P., et al., Activity-dependent isolation of the presenilin- gamma -secretase complex reveals nicastrin and a gamma substrate. Proc Natl Acad Sci U S A, 2002. 26: p. 26.
10. Wahrle, S., et al., Cholesterol-Dependent gamma-Secretase Activity in Buoyant Cholesterol- Rich Membrane Microdomains. Neurobiol Dis, 2002. 9(1): p. 11-23.
11. Kamal, A., et al., Kinesin-mediated axonal transport of a membrane compartment containing beta-secretase and presenilin-1 requires APP. Nature, 2001. 414(6864): p. 643-8.
12. Murphy, M.P., et al., gamma-Secretase, evidence for multiple proteolytic activities and influence of membrane positioning of substrate on generation of amyloid beta peptides of varying length. J Biol Chem, 1999. 274(17): p. 11914-23.
13. De Strooper, B., et al., Deficiency of presenilin-1 inhibits the normal cleavage of amyloid precursor protein [see comments]. Nature, 1998. 391(6665): p. 387-90.
14. Herreman, A., et al., Total inactivation of gamma-secretase activity in presenilin-deficient embryonic stem cells. Nat Cell Biol, 2000. 2(7): p. 461-2.
15. Zhang, Z., et al., Presenilins are required for gamma-secretase cleavage of beta-APP and transmembrane cleavage of Notch-1. Nat Cell Biol, 2000. 2(7): p. 463-5.
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