These two elegant studies by Barbara Hempstead, Bai Lu, and colleagues on brain-derived neurotrophic factor (BDNF) clearly demonstrate that both proBDNF and mature BDNF (mBDNF) can be released from neurons in culture. Which form gets released is an important question in basic neuroscience and potentially also in neurodegeneration, because, similarly to proNGF and NGF, pro- and mature BDNF activate different receptors. Their respective signalling consequence in the target neuron can be as different as attenuating or enhancing synaptic transmission, or even promoting cell death or survival. The Yang and Nagappan studies are complementary, but both are in disagreement with previous data of Matsumoto et al. (Matsumoto et al., 2008). This group had reported that cultured hippocampal neurons (derived from BDNF-myc knock-in mice) stored and secreted mBDNF but not proBDNF. However, over the last years, the idea that processing of proBDNF takes place extracellularly following the activity-dependent secretion of proBDNF from neurons has gained momentum, and these latest reports strongly support this notion.
To facilitate the detection of proBDNF and mBDNF at extremely low abundance, the authors of Yang et al. generated a knock-in mouse in which the coding exon of the endogenous BDNF gene was replaced by a C-terminal HA-tagged exon (hemagglutinin epitope tag). The authors showed that proBDNF was released from cultured neurons prepared from these mice, both if cultures were devoid of glial cells or in mixed cultures in the presence of a plasmin inhibitor. Both proBDNF and mBDNF release was increased in response to K+ depolarization of neurons. Yang et al. also reported that proBDNF levels as well those of its receptor p75 are developmentally regulated, being high prenatally and declining in adulthood.
In the second study, Nagappan et al. demonstrated that low-frequency stimulation induced predominantly proBDNF secretion from cultured neurons. By contrast, high-frequency stimulation (HFS) preferentially increased extracellular mBDNF and also the secretion of tissue plasminogen activator (tPA), a key protease involved in the extracellular conversion of proBDNF to mBDNF. These authors showed that after HFS, intracellular tPA localizes to dendritic spines and that HFS-induced increase in extracellular mBDNF occurred in dendrites. Thus, the majority of BDNF secreted by the regulated secretory pathway in response to neuronal activation is proBDNF, which is then converted to mBDNF by extracellular cleavage.
One important challenge now is to determine whether proBDNF is also released in vivo, i.e., in the hippocampus, and if its release is more abundant in aged animals or in Alzheimer disease animal models. It should be kept in mind that glial cells represent more than half of total cells in the brain (Pope, 1978) and that glia are able to rapidly process proBDNF to BDNF. Thus, measurements of basal or stimulated proBDNF release in vivo will help the field determine the physiological relevance of these new findings.
Therefore, if it can be demonstrated that the release of proBDNF shown in these two papers also occurs in vivo, then peptidase activators could become a promising therapeutic avenue for reducing extracellular concentrations of proBDNF in some pathologies where it can act as an apoptotic agent. Regulation of the expression or activation of specific proteases in particular physiological or pathological conditions (stress, aging, neurodegeneration, inflammation, injury) could therefore be extremely important in determining pro- or antiapoptotic cellular responses. Given the opposite biological effects of proBDNF and mBDNF, as well as the protective effect of BDNF against Aβ-induced toxicity in vitro and in vivo (Arancibia et al., 2008; Tapia-Arancibia et al., 2008), the possibility of modifying the ratio of mBDNF/proBDNF in order to increase cellular mBDNF availability is an important issue. The positive effect of BDNF on memory formation (Barnes and Thomas, 2008), a process impaired in neurodegenerative diseases, further reinforces this point.
Jacobsen et al. (Jacobsen et al., 2008) documented the stimulatory effects on tPA activity of the brain-penetrant small molecule (PAZ-417). It inhibits PAI-1, the endogenous inhibitor of tPA. Because Aβ40 and Aβ42 are substrates for plasmin, PAZ-417 lowered brain and plasma levels of Aβ peptides by increasing their catabolism. Although BDNF or proBDNF were not measured in this study, it is possible that PAZ-417 works doubly, increasing catabolism of Aβ peptides and also increasing proBDNF conversion to BDNF. One finding that suggests this might be the case is that high concentrations (30 or 100 mg/kg) of PAZ-417 decreased only around 20-25 percent of Aβ peptides accumulated in the brain, but it completely reversed LTP and cognitive deficits in transgenic AD mice.
As a number of proteases (neprilysin, insulin-degrading enzyme, endothelin-converting enzyme, and plasmin) have also been implicated in the proteolytic clearance of Aβ in the CNS, the exploration of these enzymatic pathways is also worthy of development.
See also:
Pope A. Neuroglia, quantitative aspects. In E. Schoffeniels, G. Franck, L. Hertz and D.B. Tower (Eds). Dynamic Properties of Glial Cells. Pergamon, Oxford, 1978, pp 13-20.
References:
Matsumoto T, Rauskolb S, Polack M, Klose J, Kolbeck R, Korte M, Barde YA.
Biosynthesis and processing of endogenous BDNF: CNS neurons store and secrete BDNF, not pro-BDNF.
Nat Neurosci. 2008 Feb;11(2):131-3.
PubMed.
Peng S, Wuu J, Mufson EJ, Fahnestock M.
Precursor form of brain-derived neurotrophic factor and mature brain-derived neurotrophic factor are decreased in the pre-clinical stages of Alzheimer's disease.
J Neurochem. 2005 Jun;93(6):1412-21.
PubMed.
Michalski B, Fahnestock M.
Pro-brain-derived neurotrophic factor is decreased in parietal cortex in Alzheimer's disease.
Brain Res Mol Brain Res. 2003 Mar 17;111(1-2):148-54.
PubMed.
Silhol M, Arancibia S, Maurice T, Tapia-Arancibia L.
Spatial memory training modifies the expression of brain-derived neurotrophic factor tyrosine kinase receptors in young and aged rats.
Neuroscience. 2007 May 25;146(3):962-73.
PubMed.
Givalois L, Arancibia S, Alonso G, Tapia-Arancibia L.
Expression of brain-derived neurotrophic factor and its receptors in the median eminence cells with sensitivity to stress.
Endocrinology. 2004 Oct;145(10):4737-47.
PubMed.
Arancibia S, Silhol M, Moulière F, Meffre J, Höllinger I, Maurice T, Tapia-Arancibia L.
Protective effect of BDNF against beta-amyloid induced neurotoxicity in vitro and in vivo in rats.
Neurobiol Dis. 2008 Sep;31(3):316-26.
PubMed.
Tapia-Arancibia L, Aliaga E, Silhol M, Arancibia S.
New insights into brain BDNF function in normal aging and Alzheimer disease.
Brain Res Rev. 2008 Nov;59(1):201-20.
PubMed.
Barnes P, Thomas KL.
Proteolysis of proBDNF is a key regulator in the formation of memory.
PLoS One. 2008;3(9):e3248.
PubMed.
Jacobsen JS, Comery TA, Martone RL, Elokdah H, Crandall DL, Oganesian A, Aschmies S, Kirksey Y, Gonzales C, Xu J, Zhou H, Atchison K, Wagner E, Zaleska MM, Das I, Arias RL, Bard J, Riddell D, Gardell SJ, Abou-Gharbia M, Robichaud A, Magolda R, Vlasuk GP, Bjornsson T, Reinhart PH, Pangalos MN.
Enhanced clearance of Abeta in brain by sustaining the plasmin proteolysis cascade.
Proc Natl Acad Sci U S A. 2008 Jun 24;105(25):8754-9.
PubMed.
These two papers from the Lu and Hempstead labs provide a thorough and interesting set of mechanistic experiments dealing with the longstanding observations that proBDNF is sorted through a regulated secretory pathway and is released primarily without cleavage in an activity-dependent fashion (Mowla et al., 1999). Previous studies by the Hempstead and Lu groups demonstrated that proBDNF induces LTD via the p75NTR receptor (Woo et al., 2005), and that tPA, which activates plasmin for conversion of proBDNF to mature BDNF, is critical for hippocampal late-phase LTP (Pang et al., 2004).
The articles under discussion here use unique reagents, antibodies specific for proBDNF and mature BDNF, and an epitope-tagged BDNF knock-in mouse, to describe how activity regulates the secretion of proBDNF and its processing to the mature form of BDNF. The Nagappan article provides novel information demonstrating that while low- and high-frequency stimulation increase secretion of proBDNF, high-frequency stimulation induces tPA secretion resulting in the extracellular processing of proBDNF to mature BDNF. Thus, differential frequencies modulate the balance of proBDNF and BDNF within the extracellular space. It is most interesting that activation of the tPA-related metalloprotease pathway also plays a role in the formation and degradation of NGF (Bruno and Cuello, 2006), suggesting a convergent pathway for the expression and regulation of different members of the NGF family of neurotrophins. However, the lack of detectable mature NGF in normal human brain (Fahnestock et al., 2001) indicates rapid in vivo degradation of mature NGF, which does not appear to be the case for mature BDNF.
BDNF and proBDNF protein levels are reduced in Alzheimer disease (AD) (Michalski and Fahnestock, 2003; Peng et al., 2005). It is therefore relevant to ask how the findings from the Lu and Hempstead labs relate to the disease process. Decreased BDNF transcription (Holsinger et al., 2000) may result in decreased proBDNF synthesis, making less proBDNF available for conversion to BDNF and resulting in attenuated signaling. This may set up a self-perpetuating spiral: reduced BDNF signaling may decrease synaptic potentiation, resulting in less neuronal activation, further reductions in proBDNF and tPA secretion, and reduced BDNF production. Reduced tPA activity in AD and increased PAI-1 are likely to further lessen BDNF levels compared to proBDNF, although this effect appears to be rather small (Peng et al., 2005).
However, this interpretation may be complicated by the observation that the high-affinity TrkB receptor for BDNF is also downregulated in AD (Salehi et al., 1996; Allen et al., 1999; Ferrer et al., 1999), with no change in the pan-neurotrophin receptor, p75NTR (Ginsberg et al., 2006). A decrease in catalytic TrkB receptor without a concomitant change in p75NTR may tip the balance towards decreased LTP and increased LTD. On the other hand, proBDNF is also capable of activating TrkB (Mowla et al., 2001; Fayard et al., 2005). Therefore, the reduced signaling of one or both BDNF isoforms through TrkB may contribute to the AD process and, along with the balance of proBDNF to BDNF, should be included in the equation when considering changes in the cellular milieu due to disease or other biological processes.
References:
Mowla SJ, Pareek S, Farhadi HF, Petrecca K, Fawcett JP, Seidah NG, Morris SJ, Sossin WS, Murphy RA.
Differential sorting of nerve growth factor and brain-derived neurotrophic factor in hippocampal neurons.
J Neurosci. 1999 Mar 15;19(6):2069-80.
PubMed.
Woo NH, Teng HK, Siao CJ, Chiaruttini C, Pang PT, Milner TA, Hempstead BL, Lu B.
Activation of p75NTR by proBDNF facilitates hippocampal long-term depression.
Nat Neurosci. 2005 Aug;8(8):1069-77.
PubMed.
Pang PT, Teng HK, Zaitsev E, Woo NT, Sakata K, Zhen S, Teng KK, Yung WH, Hempstead BL, Lu B.
Cleavage of proBDNF by tPA/plasmin is essential for long-term hippocampal plasticity.
Science. 2004 Oct 15;306(5695):487-91.
PubMed.
Bruno MA, Cuello AC.
Activity-dependent release of precursor nerve growth factor, conversion to mature nerve growth factor, and its degradation by a protease cascade.
Proc Natl Acad Sci U S A. 2006 Apr 25;103(17):6735-40.
PubMed.
Fahnestock M, Michalski B, Xu B, Coughlin MD.
The precursor pro-nerve growth factor is the predominant form of nerve growth factor in brain and is increased in Alzheimer's disease.
Mol Cell Neurosci. 2001 Aug;18(2):210-20.
PubMed.
Michalski B, Fahnestock M.
Pro-brain-derived neurotrophic factor is decreased in parietal cortex in Alzheimer's disease.
Brain Res Mol Brain Res. 2003 Mar 17;111(1-2):148-54.
PubMed.
Peng S, Wuu J, Mufson EJ, Fahnestock M.
Precursor form of brain-derived neurotrophic factor and mature brain-derived neurotrophic factor are decreased in the pre-clinical stages of Alzheimer's disease.
J Neurochem. 2005 Jun;93(6):1412-21.
PubMed.
Holsinger RM, Schnarr J, Henry P, Castelo VT, Fahnestock M.
Quantitation of BDNF mRNA in human parietal cortex by competitive reverse transcription-polymerase chain reaction: decreased levels in Alzheimer's disease.
Brain Res Mol Brain Res. 2000 Mar 29;76(2):347-54.
PubMed.
Salehi A, Verhaagen J, Dijkhuizen PA, Swaab DF.
Co-localization of high-affinity neurotrophin receptors in nucleus basalis of Meynert neurons and their differential reduction in Alzheimer's disease.
Neuroscience. 1996 Nov;75(2):373-87.
PubMed.
Allen SJ, Wilcock GK, Dawbarn D.
Profound and selective loss of catalytic TrkB immunoreactivity in Alzheimer's disease.
Biochem Biophys Res Commun. 1999 Nov 2;264(3):648-51.
PubMed.
Ferrer I, Marín C, Rey MJ, Ribalta T, Goutan E, Blanco R, Tolosa E, Martí E.
BDNF and full-length and truncated TrkB expression in Alzheimer disease. Implications in therapeutic strategies.
J Neuropathol Exp Neurol. 1999 Jul;58(7):729-39.
PubMed.
Ginsberg SD, Che S, Wuu J, Counts SE, Mufson EJ.
Down regulation of trk but not p75NTR gene expression in single cholinergic basal forebrain neurons mark the progression of Alzheimer's disease.
J Neurochem. 2006 Apr;97(2):475-87.
PubMed.
Mowla SJ, Farhadi HF, Pareek S, Atwal JK, Morris SJ, Seidah NG, Murphy RA.
Biosynthesis and post-translational processing of the precursor to brain-derived neurotrophic factor.
J Biol Chem. 2001 Apr 20;276(16):12660-6.
PubMed.
Fayard B, Loeffler S, Weis J, Vögelin E, Krüttgen A.
The secreted brain-derived neurotrophic factor precursor pro-BDNF binds to TrkB and p75NTR but not to TrkA or TrkC.
J Neurosci Res. 2005 Apr 1;80(1):18-28.
PubMed.
Comments
Université Montpellier 2
These two elegant studies by Barbara Hempstead, Bai Lu, and colleagues on brain-derived neurotrophic factor (BDNF) clearly demonstrate that both proBDNF and mature BDNF (mBDNF) can be released from neurons in culture. Which form gets released is an important question in basic neuroscience and potentially also in neurodegeneration, because, similarly to proNGF and NGF, pro- and mature BDNF activate different receptors. Their respective signalling consequence in the target neuron can be as different as attenuating or enhancing synaptic transmission, or even promoting cell death or survival. The Yang and Nagappan studies are complementary, but both are in disagreement with previous data of Matsumoto et al. (Matsumoto et al., 2008). This group had reported that cultured hippocampal neurons (derived from BDNF-myc knock-in mice) stored and secreted mBDNF but not proBDNF. However, over the last years, the idea that processing of proBDNF takes place extracellularly following the activity-dependent secretion of proBDNF from neurons has gained momentum, and these latest reports strongly support this notion.
To facilitate the detection of proBDNF and mBDNF at extremely low abundance, the authors of Yang et al. generated a knock-in mouse in which the coding exon of the endogenous BDNF gene was replaced by a C-terminal HA-tagged exon (hemagglutinin epitope tag). The authors showed that proBDNF was released from cultured neurons prepared from these mice, both if cultures were devoid of glial cells or in mixed cultures in the presence of a plasmin inhibitor. Both proBDNF and mBDNF release was increased in response to K+ depolarization of neurons. Yang et al. also reported that proBDNF levels as well those of its receptor p75 are developmentally regulated, being high prenatally and declining in adulthood.
In the second study, Nagappan et al. demonstrated that low-frequency stimulation induced predominantly proBDNF secretion from cultured neurons. By contrast, high-frequency stimulation (HFS) preferentially increased extracellular mBDNF and also the secretion of tissue plasminogen activator (tPA), a key protease involved in the extracellular conversion of proBDNF to mBDNF. These authors showed that after HFS, intracellular tPA localizes to dendritic spines and that HFS-induced increase in extracellular mBDNF occurred in dendrites. Thus, the majority of BDNF secreted by the regulated secretory pathway in response to neuronal activation is proBDNF, which is then converted to mBDNF by extracellular cleavage.
One important challenge now is to determine whether proBDNF is also released in vivo, i.e., in the hippocampus, and if its release is more abundant in aged animals or in Alzheimer disease animal models. It should be kept in mind that glial cells represent more than half of total cells in the brain (Pope, 1978) and that glia are able to rapidly process proBDNF to BDNF. Thus, measurements of basal or stimulated proBDNF release in vivo will help the field determine the physiological relevance of these new findings.
In AD patients, both proBDNF and mBDNF are decreased in the parietal cortex and hippocampus even in preclinical stages (Peng et al., 2005; Michalski and Fahnestock, 2003). In contrast, we have reported that proBDNF levels are increased in aged rat hippocampus (Silhol et al., 2007). We also measured BDNF release from hypothalamus of adult rats under stress conditions (Givalois et al., 2004; Arancibia et al., 2007) or from posterior cingular cortex in vivo (Arancibia et al., 2008) using push-pull perfusion experiments.
Therefore, if it can be demonstrated that the release of proBDNF shown in these two papers also occurs in vivo, then peptidase activators could become a promising therapeutic avenue for reducing extracellular concentrations of proBDNF in some pathologies where it can act as an apoptotic agent. Regulation of the expression or activation of specific proteases in particular physiological or pathological conditions (stress, aging, neurodegeneration, inflammation, injury) could therefore be extremely important in determining pro- or antiapoptotic cellular responses. Given the opposite biological effects of proBDNF and mBDNF, as well as the protective effect of BDNF against Aβ-induced toxicity in vitro and in vivo (Arancibia et al., 2008; Tapia-Arancibia et al., 2008), the possibility of modifying the ratio of mBDNF/proBDNF in order to increase cellular mBDNF availability is an important issue. The positive effect of BDNF on memory formation (Barnes and Thomas, 2008), a process impaired in neurodegenerative diseases, further reinforces this point.
Jacobsen et al. (Jacobsen et al., 2008) documented the stimulatory effects on tPA activity of the brain-penetrant small molecule (PAZ-417). It inhibits PAI-1, the endogenous inhibitor of tPA. Because Aβ40 and Aβ42 are substrates for plasmin, PAZ-417 lowered brain and plasma levels of Aβ peptides by increasing their catabolism. Although BDNF or proBDNF were not measured in this study, it is possible that PAZ-417 works doubly, increasing catabolism of Aβ peptides and also increasing proBDNF conversion to BDNF. One finding that suggests this might be the case is that high concentrations (30 or 100 mg/kg) of PAZ-417 decreased only around 20-25 percent of Aβ peptides accumulated in the brain, but it completely reversed LTP and cognitive deficits in transgenic AD mice.
As a number of proteases (neprilysin, insulin-degrading enzyme, endothelin-converting enzyme, and plasmin) have also been implicated in the proteolytic clearance of Aβ in the CNS, the exploration of these enzymatic pathways is also worthy of development.
See also:
Pope A. Neuroglia, quantitative aspects. In E. Schoffeniels, G. Franck, L. Hertz and D.B. Tower (Eds). Dynamic Properties of Glial Cells. Pergamon, Oxford, 1978, pp 13-20.
References:
Matsumoto T, Rauskolb S, Polack M, Klose J, Kolbeck R, Korte M, Barde YA. Biosynthesis and processing of endogenous BDNF: CNS neurons store and secrete BDNF, not pro-BDNF. Nat Neurosci. 2008 Feb;11(2):131-3. PubMed.
Peng S, Wuu J, Mufson EJ, Fahnestock M. Precursor form of brain-derived neurotrophic factor and mature brain-derived neurotrophic factor are decreased in the pre-clinical stages of Alzheimer's disease. J Neurochem. 2005 Jun;93(6):1412-21. PubMed.
Michalski B, Fahnestock M. Pro-brain-derived neurotrophic factor is decreased in parietal cortex in Alzheimer's disease. Brain Res Mol Brain Res. 2003 Mar 17;111(1-2):148-54. PubMed.
Silhol M, Arancibia S, Maurice T, Tapia-Arancibia L. Spatial memory training modifies the expression of brain-derived neurotrophic factor tyrosine kinase receptors in young and aged rats. Neuroscience. 2007 May 25;146(3):962-73. PubMed.
Givalois L, Arancibia S, Alonso G, Tapia-Arancibia L. Expression of brain-derived neurotrophic factor and its receptors in the median eminence cells with sensitivity to stress. Endocrinology. 2004 Oct;145(10):4737-47. PubMed.
Arancibia S, Silhol M, Moulière F, Meffre J, Höllinger I, Maurice T, Tapia-Arancibia L. Protective effect of BDNF against beta-amyloid induced neurotoxicity in vitro and in vivo in rats. Neurobiol Dis. 2008 Sep;31(3):316-26. PubMed.
Tapia-Arancibia L, Aliaga E, Silhol M, Arancibia S. New insights into brain BDNF function in normal aging and Alzheimer disease. Brain Res Rev. 2008 Nov;59(1):201-20. PubMed.
Barnes P, Thomas KL. Proteolysis of proBDNF is a key regulator in the formation of memory. PLoS One. 2008;3(9):e3248. PubMed.
Jacobsen JS, Comery TA, Martone RL, Elokdah H, Crandall DL, Oganesian A, Aschmies S, Kirksey Y, Gonzales C, Xu J, Zhou H, Atchison K, Wagner E, Zaleska MM, Das I, Arias RL, Bard J, Riddell D, Gardell SJ, Abou-Gharbia M, Robichaud A, Magolda R, Vlasuk GP, Bjornsson T, Reinhart PH, Pangalos MN. Enhanced clearance of Abeta in brain by sustaining the plasmin proteolysis cascade. Proc Natl Acad Sci U S A. 2008 Jun 24;105(25):8754-9. PubMed.
McMaster University
These two papers from the Lu and Hempstead labs provide a thorough and interesting set of mechanistic experiments dealing with the longstanding observations that proBDNF is sorted through a regulated secretory pathway and is released primarily without cleavage in an activity-dependent fashion (Mowla et al., 1999). Previous studies by the Hempstead and Lu groups demonstrated that proBDNF induces LTD via the p75NTR receptor (Woo et al., 2005), and that tPA, which activates plasmin for conversion of proBDNF to mature BDNF, is critical for hippocampal late-phase LTP (Pang et al., 2004).
The articles under discussion here use unique reagents, antibodies specific for proBDNF and mature BDNF, and an epitope-tagged BDNF knock-in mouse, to describe how activity regulates the secretion of proBDNF and its processing to the mature form of BDNF. The Nagappan article provides novel information demonstrating that while low- and high-frequency stimulation increase secretion of proBDNF, high-frequency stimulation induces tPA secretion resulting in the extracellular processing of proBDNF to mature BDNF. Thus, differential frequencies modulate the balance of proBDNF and BDNF within the extracellular space. It is most interesting that activation of the tPA-related metalloprotease pathway also plays a role in the formation and degradation of NGF (Bruno and Cuello, 2006), suggesting a convergent pathway for the expression and regulation of different members of the NGF family of neurotrophins. However, the lack of detectable mature NGF in normal human brain (Fahnestock et al., 2001) indicates rapid in vivo degradation of mature NGF, which does not appear to be the case for mature BDNF.
BDNF and proBDNF protein levels are reduced in Alzheimer disease (AD) (Michalski and Fahnestock, 2003; Peng et al., 2005). It is therefore relevant to ask how the findings from the Lu and Hempstead labs relate to the disease process. Decreased BDNF transcription (Holsinger et al., 2000) may result in decreased proBDNF synthesis, making less proBDNF available for conversion to BDNF and resulting in attenuated signaling. This may set up a self-perpetuating spiral: reduced BDNF signaling may decrease synaptic potentiation, resulting in less neuronal activation, further reductions in proBDNF and tPA secretion, and reduced BDNF production. Reduced tPA activity in AD and increased PAI-1 are likely to further lessen BDNF levels compared to proBDNF, although this effect appears to be rather small (Peng et al., 2005).
However, this interpretation may be complicated by the observation that the high-affinity TrkB receptor for BDNF is also downregulated in AD (Salehi et al., 1996; Allen et al., 1999; Ferrer et al., 1999), with no change in the pan-neurotrophin receptor, p75NTR (Ginsberg et al., 2006). A decrease in catalytic TrkB receptor without a concomitant change in p75NTR may tip the balance towards decreased LTP and increased LTD. On the other hand, proBDNF is also capable of activating TrkB (Mowla et al., 2001; Fayard et al., 2005). Therefore, the reduced signaling of one or both BDNF isoforms through TrkB may contribute to the AD process and, along with the balance of proBDNF to BDNF, should be included in the equation when considering changes in the cellular milieu due to disease or other biological processes.
References:
Mowla SJ, Pareek S, Farhadi HF, Petrecca K, Fawcett JP, Seidah NG, Morris SJ, Sossin WS, Murphy RA. Differential sorting of nerve growth factor and brain-derived neurotrophic factor in hippocampal neurons. J Neurosci. 1999 Mar 15;19(6):2069-80. PubMed.
Woo NH, Teng HK, Siao CJ, Chiaruttini C, Pang PT, Milner TA, Hempstead BL, Lu B. Activation of p75NTR by proBDNF facilitates hippocampal long-term depression. Nat Neurosci. 2005 Aug;8(8):1069-77. PubMed.
Pang PT, Teng HK, Zaitsev E, Woo NT, Sakata K, Zhen S, Teng KK, Yung WH, Hempstead BL, Lu B. Cleavage of proBDNF by tPA/plasmin is essential for long-term hippocampal plasticity. Science. 2004 Oct 15;306(5695):487-91. PubMed.
Bruno MA, Cuello AC. Activity-dependent release of precursor nerve growth factor, conversion to mature nerve growth factor, and its degradation by a protease cascade. Proc Natl Acad Sci U S A. 2006 Apr 25;103(17):6735-40. PubMed.
Fahnestock M, Michalski B, Xu B, Coughlin MD. The precursor pro-nerve growth factor is the predominant form of nerve growth factor in brain and is increased in Alzheimer's disease. Mol Cell Neurosci. 2001 Aug;18(2):210-20. PubMed.
Michalski B, Fahnestock M. Pro-brain-derived neurotrophic factor is decreased in parietal cortex in Alzheimer's disease. Brain Res Mol Brain Res. 2003 Mar 17;111(1-2):148-54. PubMed.
Peng S, Wuu J, Mufson EJ, Fahnestock M. Precursor form of brain-derived neurotrophic factor and mature brain-derived neurotrophic factor are decreased in the pre-clinical stages of Alzheimer's disease. J Neurochem. 2005 Jun;93(6):1412-21. PubMed.
Holsinger RM, Schnarr J, Henry P, Castelo VT, Fahnestock M. Quantitation of BDNF mRNA in human parietal cortex by competitive reverse transcription-polymerase chain reaction: decreased levels in Alzheimer's disease. Brain Res Mol Brain Res. 2000 Mar 29;76(2):347-54. PubMed.
Salehi A, Verhaagen J, Dijkhuizen PA, Swaab DF. Co-localization of high-affinity neurotrophin receptors in nucleus basalis of Meynert neurons and their differential reduction in Alzheimer's disease. Neuroscience. 1996 Nov;75(2):373-87. PubMed.
Allen SJ, Wilcock GK, Dawbarn D. Profound and selective loss of catalytic TrkB immunoreactivity in Alzheimer's disease. Biochem Biophys Res Commun. 1999 Nov 2;264(3):648-51. PubMed.
Ferrer I, Marín C, Rey MJ, Ribalta T, Goutan E, Blanco R, Tolosa E, Martí E. BDNF and full-length and truncated TrkB expression in Alzheimer disease. Implications in therapeutic strategies. J Neuropathol Exp Neurol. 1999 Jul;58(7):729-39. PubMed.
Ginsberg SD, Che S, Wuu J, Counts SE, Mufson EJ. Down regulation of trk but not p75NTR gene expression in single cholinergic basal forebrain neurons mark the progression of Alzheimer's disease. J Neurochem. 2006 Apr;97(2):475-87. PubMed.
Mowla SJ, Farhadi HF, Pareek S, Atwal JK, Morris SJ, Seidah NG, Murphy RA. Biosynthesis and post-translational processing of the precursor to brain-derived neurotrophic factor. J Biol Chem. 2001 Apr 20;276(16):12660-6. PubMed.
Fayard B, Loeffler S, Weis J, Vögelin E, Krüttgen A. The secreted brain-derived neurotrophic factor precursor pro-BDNF binds to TrkB and p75NTR but not to TrkA or TrkC. J Neurosci Res. 2005 Apr 1;80(1):18-28. PubMed.