Protection against Fatal Sindbis Virus Encephalitis by Beclin, a Novel Bcl-2-Interacting Protein

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Liang, X. H.
	Articles by Levine, B.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Liang, X. H.
	Articles by Levine, B.

Journal of Virology, November 1998, p. 8586-8596, Vol. 72, No. 11
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Protection against Fatal Sindbis Virus Encephalitis by Beclin, a Novel Bcl-2-Interacting Protein

Xiao Huan Liang,¹ Linda K. Kleeman,¹ Hui Hui Jiang, Gerald Gordon,² James E. Goldman,³ Gail Berry,² Brian Herman,²^, and Beth Levine¹^,^*

Departments of Medicine¹ and Pathology,³ Columbia University College of Physicians and Surgeons, New York, New York 10032, and Department of Cell Biology and Anatomy, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599²

Received 5 May 1998/Accepted 6 July 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

bcl-2, the prototypic cellular antiapoptotic gene, decreases Sindbis virus replication and Sindbis virus-induced apoptosisin mouse brains, resulting in protection against lethal encephalitis.To investigate potential mechanisms by which Bcl-2 protects againstcentral nervous system Sindbis virus infection, we performed ayeast two-hybrid screen to identify Bcl-2-interacting gene productsin an adult mouse brain library. We identified a novel 60-kDacoiled-coil protein, Beclin, which we confirmed interacts withBcl-2 in mammalian cells, using fluorescence resonance energytransfer microscopy. To examine the role of Beclin in Sindbisvirus pathogenesis, we constructed recombinant Sindbis virus chimerasthat express full-length human Beclin (SIN/beclin), Beclin lackingthe putative Bcl-2-binding domain (SIN/beclin $Delta$ Bcl-2BD), or Beclincontaining a premature stop codon near the 5' terminus (SIN/beclinstop).The survival of mice infected with SIN/beclin was significantlyhigher (71%) than the survival of mice infected with SIN/beclin $Delta$ Bcl-2BD(9%) or SIN/beclinstop (7%) (P < 0.001). The brains of mice infectedwith SIN/beclin had fewer Sindbis virus RNA-positive cells, fewerapoptotic cells, and lower viral titers than the brains of miceinfected with SIN/beclin $Delta$ Bcl-2BD or SIN/beclinstop. These findingsdemonstrate that Beclin is a novel Bcl-2-interacting cellularprotein that may play a role in antiviral host defense.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The cellular antiapoptotic gene bcl-2 represents a novel class of antiviral host defense molecules which function both byrestricting viral replication and by preventing virus-inducedcell death. Bcl-2 blocks apoptosis in vitro induced by severaldifferent RNA viruses, including Sindbis virus (18, 41), influenzavirus (13, 26), reovirus (31), Semliki Forest virus (34),LaCrosse virus (29), and Japanese B encephalitis virus (21).Previously, we have shown that Bcl-2 overexpression in virallyinfected neurons in vivo also protects mice against fatal encephalitiscaused by the prototypic alphavirus, Sindbis virus (17). Theprotective effects of Bcl-2 against fatal Sindbis virus encephalitiswere associated with a reduction both in neuronal apoptotic deathand in central nervous system (CNS) viral replication. A similarantiviral effect of Bcl-2 overexpression has been observed duringSindbis virus infection in cultured AT3 cells (41) as well asduring influenza virus infection of MDCK cells (26), JapaneseB encephalitis virus infection of N18 cells (21), and SemlikiForest virus infection of AT3 cells (34). Although the roleof endogenous Bcl-2 in antiviral defense has yet to be evaluated,these studies support the hypothesis that Bcl-2 may be importantin protecting cells against viral infections.

Most previous studies examining the effects of Bcl-2 on viral infections have been with neurotropic RNA viruses (e.g., Sindbisvirus, reovirus, Semliki Forest virus, LaCrosse virus, and JapaneseB virus) (18, 21, 29, 31, 34, 41). Although Bcl-2may affect viral replication and virus-induced apoptosis withnonneurotropic viruses (e.g., influenza virus) (13, 26), hostmech-anisms to inhibit apoptosis may be of particular importanceduring viral infections of vital, nonrenewable cell populationssuch as neurons. In such instances, virus-induced apoptotic deathof neurons may result in irreversible CNS pathology and deathof the host organism (1, 17, 19, 25). Therefore, whileapoptosis in other cell types may be an adaptive host defensestrategy that reduces total viral burden for the organism (reviewedin references 11, 16, 36, and 39), unique strategies mayhave evolved to permit control of CNS viral replication withoutinducing apoptotic death of infected neurons. It is thus possiblethat cellular genes that play a role in preventing apoptosis duringnormal neuronal development (e.g., bcl-2 and bcl-x_L) (reviewedin reference 23) may also be important in regulating CNS viralreplication and in defending against apoptosis induced by neurotropicviruses.

To further understand how the cellular gene bcl-2 exerts antiapoptotic and antiviral effects during CNS viral infection, weperformed a yeast two-hybrid screen to identify Bcl-2-interactinggene products in adult mouse brain. In this study, we describethe identification of a novel Bcl-2-interacting gene product,which we named Beclin because of its predicted coiled-coil structure(hence, the "-in" suffix) and its interaction with Bcl-2 (Becl).Like Bcl-2 overexpression, Beclin overexpression in neurons invivo can inhibit Sindbis virus replication, reduce CNS apoptosis,and provide protection against fatal Sindbis virus infection.A Beclin construct lacking the putative Bcl-2-binding domain providesno protection and has no antiviral activity. Thus, our findingsidentify a novel protein, Beclin, which may play a role in hostdefense against Sindbis virus infection. In addition, they suggestthat interactions with Bcl-2-like proteins may be important forthe protective activity of Beclin.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Plasmids. To construct vectors for transient expression in mammalian cells, the open reading frame of human bcl-2, flag epitope-taggedhuman beclin, and flag epitope-tagged beclin deleted of nucleotides238 to 453 were cloned into pSG5 (Stratagene). To construct viralcDNA clones, the previously described neurovirulent double subgenomicSindbis virus vector dsTE12 was used (17). Full-length flagepitope-tagged human beclin, human beclin containing a stop codoninserted at nucleotide position 270, human beclin containing anin-frame deletion of nucleotides 238 to 453, human bcl-2, andhuman bcl-2 containing a stop codon at nucleotide position 118were cloned into the BstEII site of dsTE12 to generate plasmidsSIN/beclin, SIN/beclinstop, SIN/beclin $Delta$ bcl-2BD, SIN/bcl-2, andSIN/bcl-2stop, respectively. To construct vectors for yeast two-hybridstudies, the sequences encoding amino acids (aa) 1 to 218 of humanbcl-2, 1 to 212 of bcl-x_L, 1 to 149 of bcl-x_S, and 1 to 171 ofbax were cloned into pGBT9 in frame with the GAL4 DNA-bindingdomain. To avoid difficulties with targeting of proteins to thenucleus, the sequences encoding C-terminal transmembrane domainsof bcl-2 family members were omitted. Control pGBT9 plasmids containinglamin (pLAM5') and p53 (pVA3) inserts were obtained from Clontech.

Yeast two-hybrid screen. Saccharomyces cerevisiae SFY526 cells were cotransformed with pGBT9/bcl-2 and 10⁶ cDNA molecules from an adult mouse brain library fused to a GAL4activation domain vector (pGAD10; Clontech), plated onto SD mediumlacking tryptophan and leucine, incubated at 30°C for 4 days,and then screened for LacZ activity by a colony lift filter assay.Putative interacting clones were isolated by manipulation in leuBEscherichia coli, and further tested against pGBT9 and controlplasmids. A positive $beta$ -galactosidase reaction between pGBT9/bcl-2and clone F1 was obtained within 10 to 15 min. For analysis ofinteractions between Beclin and Bcl-2 family members, pGBT9 plasmidscontaining bcl-2 family members were cotransformed with fragmentsof human beclin (1 to 450, 262 to 450, and 1 to 708) fused tothe GAL4 activation domain in pGAD424, and transformants werescreened for LacZ activity.

Sequencing and analysis of human beclin. The partial nucleotide sequence of mouse beclin obtained from sequencing clone F1 was aligned with an overlapping clone GT197isolated from human breast (32). Primers immediately upstreamand downstream of the predicted open reading frame were used toamplify the coding sequence of human beclin from a normalizedhuman infant brain cDNA library (37). The resulting PCR productsfrom several independent reactions were cloned into pCRII andsequenced in both directions, using Sequenase (U.S. Biochemical)as well as automated sequencing. The resulting nucleotide sequenceand deduced amino acid sequences were used to scan various databanks (GenBank, EMBL, SwissProt, and PIR) for homologous sequences,using the BLAST algorithms (2). The amino acid sequence wasalso analyzed by the PROSITE program to identify functional motifsand by the COILS program to identify coiled-coil regions (22).

Northern blot analysis. Human and mouse multiple tissue blots (Clontech) were hybridized with ³²P randomly labeled human or mouse beclin probes (nucleotides 1to 485) as instructed by the manufacturer (Clontech). Equal loading[2 µg of poly(A) RNA] was confirmed by hybridization to a $beta$ -actinprobe.

Production of recombinant viruses. The viruses SIN/beclin, SIN/beclinstop, SIN/beclin $Delta$ Bcl-2BD, SIN/bcl-2, and SIN/bcl-2stop were generated from viral cDNA clonesas previously described (17). Briefly, 5'-capped transcriptswere synthesized from cDNA clones linearized with PvuI (for beclin-containingviruses) or XhoI (for bcl-2-containing viruses), transcribed invitro with SP6 DNA-dependent RNA polymerase, and transfected intoBHK cells by using Lipofectin according to the manufacturer'sinstructions. Twenty-four hours after transfection, virus particle-containingsupernatants of transfected cell monolayers were collected, frozenin aliquots at 70°C, and used for all subsequent experiments.Titers of stock viruses were determined by plaque assay titrationon BHK-21 cells.

Animal experiments. Ten-day-old litters of CD1 mice were inoculated intracerebrally into the right cerebral hemisphere with 1,000 PFU of eachrecombinant virus in 0.03 ml of Hanks' balanced salt solution.For mortality experiments, three to six separate litters wereinoculated with each virus, and mortality was determined by dailyobservation of the mice for 3 weeks after infection. For virustitration and histopathology experiments, three to six mice perexperimental group were sacrificed at days 1, 2, and 4 after inoculation.The right cerebral hemisphere was dissected and stored at $-$ 70°C,and freeze-thawed tissues were used to prepare 10% homogenatesin Hanks' balanced salt solution for plaque assay titration. Theleft cerebral hemisphere was fixed by immersion in 3% paraformaldehyde.

Histopathology. Paraformaldehyde-fixed mouse brains were embedded in paraffin, and a series of 4-µm parasagittal sections were cut at thelevel of the olfactory bulb, extending caudally from the bulbto the cerebellum and medulla. For each brain, sequential sectionswere stained by hematoxylin and eosin to detect histopathology,in situ end labeling (ISEL) to detect apoptotic nuclei, in situhybridization to detect Sindbis virus RNA, and immunoperoxidaseto detect flag-Beclin protein expression. ISEL and in situ hybridizationwere performed by methods identical to those described previouslyfor SIN/bcl-2-infected mouse brains (17). Immunoperoxidase stainingto detect flag-Beclin protein expression in SIN/beclin-, SIN/beclin $Delta$ Bcl-2BD-,and SIN/beclinstop-infected mouse brains was performed by usingthe monoclonal anti-flag antibody M2 (5 µg/ml; VWR) and the avidin-biotinperoxidase method (Vectastain ABC kit; Vector Laboratories) accordingto the manufacturer's instructions.

The number of virus RNA-positive and ISEL-positive cells in each brain section was quantitated with Image-ProPlus software.To calculate the number of positive cells per brain section, nonoverlapping0.25-mm² microscopic fields spanning the entire brain section were scannedwith a 10× objective and constant settings for brightness, contrast,and threshold values for positive events. The number of positiveevents (i.e., RNA-positive cells or ISEL-positive cells) for eachbrain section was determined by adding the sum of all individualfields analyzed. The total number of positive events per brainsection was divided by the total area of the brain section toyield the average number of RNA-positive or ISEL-positive cellsper square millimeter of brain.

Sections of hippocampus and anterior cortex from an adult human were stained with 843, a polyclonal antibody against a humanBeclin peptide corresponding to aa 1 to 15 (1:200 dilution; Eurogenetics,Seraing, Belgium), and human Beclin was detected by the avidin-biotinperoxidase method.

Plasmid transfections. Plasmids pSG5/bcl-2 and pSG5/flag-beclin or pSG5/bcl-2 and pSG5/flag-beclin $Delta$ Bcl-2BD (1 µg of each) were transiently transfectedinto COS7 cells by using Superfect (Qiagen) according to the manufacturer'sinstructions.

Protein detection. For immunofluorescence studies, COS7 cells were fixed 24 h after transfection with 100% ethanol. Expression of flag-Beclinand flag-mutant Beclin $Delta$ Bcl-2BD mutant constructs was detectedwith an anti-flag epitope antibody (M2; 1:20; VWR) and fluoresceinisothiocyanate (FITC)-conjugated horse anti-mouse immunoglobulinG. Bcl-2 expression was detected with a polyclonal rabbit anti-Bcl-2antibody (1:100; Pharmingen) and rhodamine-conjugated goat anti-rabbitantibody. SERCA (endoplasmic reticulum Ca²⁺ ATPase) was detected with an anti-SERCA antibody (1:500; ResearchDesign, Inc.). Western blot analysis to detect flag-Beclin expressionin BHK cells infected with SIN/beclin, SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BDwas performed with either antibody M2 (20 µg/ml) or anti-humanBeclin peptide antibody 843 (1:200) and enhanced chemiluminescencedetection as instructed by the manufacturer (Amersham).

FRET. Fluorescence resonance energy transfer (FRET) microscopy was performed as previously described on COS7 cells cotransfectedwith bcl-2 and beclin expression vectors (9). The donor (FITC)filter set had the following parameters: excitation (ex) = 450to 490 nm; dichroic mirror (dm) = 510 nm; emission (em) = 590long pass. The acceptor (rhodamine) filter set had the followingparameters: ex = 546 nm; dm = 580 nm, em = 590 long pass. Imagesobtained with these two filter sets were used to directly quantifythe intensities of each fluorophore. The signal recorded fromthe FRET filter set (ex = 450 to 490 nm; dm = 580 nm; em = 590nm long pass) is from energy that has transferred from FITC torhodamine molecules. A mapping program described previously (9)was used to map fluorescent cells and to quantify the intensitywithin each cell. Quantitative analysis of these mapped imagesrequired solving three equations, one for each filter set, whichaccounted for the excitation and detection of both labels in allthree filter sets as well as the concentrations of the donor andacceptor molecules and the probability of transfer. The measuredquantities are expressed as follows, in which the first letter(uppercase) indicates the filter set (A, acceptor; F, FRET; D,donor) and the second letter (lowercase) indicates the labelspresent (a, acceptor alone; f, acceptor and donor; d, donor alone).A solution of the equation is E = 1/[aconc(RK + 1)], where aconc= (AdFf $-$ FdAf)/[(AdFa/Aa) $-$ Fd]; R = (DaFf/Fa $-$ Df)/[aconc ((Fa/Aa) $-$ FdDa/DdAa) $-$ F = FdDf/Dd]; and K is proportional to the productof the ratio of the quantum yield of the two labels and the ratioof the absolute detection efficiencies of the two labels.

Nucleotide sequence accession numbers. The GenBank accession numbers for human and mouse beclin are AF077301 and AF077302, respectively.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Identification of beclin, a novel gene on chromosome 17q21. Previously, we demonstrated that Bcl-2 inhibits Sindbis virus replication and prevents Sindbis virus-induced apoptosis inmouse neurons (17). To further understand the mechanisms bywhich Bcl-2 protects against Sindbis virus infection in neurons,we performed a yeast two-hybrid screen of an adult mouse brainlibrary for complementary DNAs encoding proteins that bind tothe cell death inhibitor Bcl-2. We constructed a bait plasmid(pGBT9/bcl-2) by fusing human bcl-2 (lacking the C-terminal signal-anchorsequence to ensure translocation to the nucleus) to the GAL4 DNA-bindingdomain, which was cotransformed with an oligo(dT) and random hexamer-primedadult mouse brain cDNA fusion library in a GAL4 activation domainvector, pGAD10. Of 1 million transformants, one positive colonywas identified by the 5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside(X-Gal) filter assay. Sequencing analysis of the cDNA plasmidrescued from this colony (F1) revealed a termination codon 42bp downstream from the GAL4 activation domain, several predictedshort open reading frames between nucleotides 124 and 1843 anda longer predicted open reading frame (with a good Kozak consensussequence and multiple stop codons upstream) spanning from nucleotide1855 to the 3' end of the insert. Thus, either the 14-aa fusionprotein was interacting with Bcl-2 or one of the downstream openreading frames encoded a protein that contains its own activationdomain and interacts with Bcl-2. To identify the Bcl-2-interactingregion of F1, we fused nucleotides 1 to 1854 and 1855 to 2500to the GAL4 activation domain in pGAD424 and tested for interactionswith Bcl-2. Nucleotides 1855 to 2500, but not 1 to 1854, encodeda protein that interacts with Bcl-2 fused to the GAL4 DNA-bindingdomain (Table 1) but not with control GAL4 DNA-binding domainplasmids containing p53, lamin (Table 1), or Sindbis virus glycoproteins(data not shown).

View this table:
[in this window]
[in a new window]

TABLE 1. Summary of yeast two-hybrid assay results

A database search revealed that the nucleotide sequence of F1 (1855 to 2500) overlapped with sequences of several clones isolatedfrom a normalized infant human brain cDNA library in the MerckEST (epitope tag sequence) database as well as clones from humanbreast (GT197) (32) and human fibroblast (B32) cells (8).These clones contain only partial open reading frames of a novelgene that encodes a protein with coiled coils. As explained above,we assigned the name beclin to this gene because of the interactionof its encoded protein with Bcl-2 and the predicted coiled-coilstructure of its encoded protein. Clones GT197 and B32 were bothisolated in the generation of transcription maps of the breastcancer susceptibility locus on chromosome 17q21 and are mappedto a region located approximately 100 kb centromeric to the geneBRCA1. They lie within a 400-kb minimal deletion unit mapped byTangir et al. in sporadic epithelial ovarian cancers (38).

We aligned the overlapping partial clones in GenBank with our mouse beclin sequence to obtain a predicted sequence of thefull-length open reading frame of human beclin and isolated humanbeclin from a normalized human infant brain cDNA library (37).Human beclin is predicted to encode a novel 450-aa, 60-kDa proteincontaining a coiled-coil region with 25 to 28% homology with myosin-likeproteins (Fig. 1). It shares 93% identity at the nucleotide leveland 98% identity at the amino acid level with the mouse beclinsequence identified in the yeast two-hybrid screen. Human Beclinis also homologous with the Caenorhabditis elegans T19E7.3 geneproduct (GenBank accession no. U42843) and the S. cerevisiaegene product Lph7p (GenBank accession no. U43503) (38 and 37%identical over 145 and 137 residues, respectively), indicatinga high degree of evolutionary conservation. PROSITE analysis ofhuman Beclin identified several potential glycosylation, phosphorylation,and myristoylation sites but no other functional sequence motifs.

View larger version (39K):
[in this window]
[in a new window]

FIG. 1. Deduced amino acid sequence of human Beclin. The boxed area represents the Bcl-2-binding domain of human Beclin (Table 1), and the underlined area corresponds to the region that is predicted to have a coiled-coil conformation.

Ubiquitous expression of beclin mRNA in mouse and human tissues. To examine the tissue-specific pattern of beclin expression, we hybridized mouse and human multiple-tissue Northern blotswith a beclin-specific probe. RNA blot analysis revealed thatexpression of beclin mRNA is widespread in both mouse and humanadult tissue (Fig. 2A). A beclin-specific probe hybridized toa 2.2-kb transcript present at highest levels in human skeletalmuscle but at detectable levels in all tissues examined. The sizeof this transcript is approximately the same as that observedpreviously for clones GT197 and B32 (8, 32). In some tissues,additional 1.7- and 1.4-kb transcripts were observed, suggestingthe presence of alternatively spliced transcripts.

View larger version (31K):
[in this window]
[in a new window]

View larger version (104K):
[in this window]
[in a new window]

FIG. 2. Beclin mRNA and protein expression. (A) Northern blot analysis of beclin mRNA expression in human and mouse tissues. sm., small; m., muscle. (B) Immunoperoxidase staining of an adult human hippocampus section with a polyclonal antibody against a human Beclin peptide. The arrow marks a Beclin-positive neuron. Magnification, ×450.

Beclin is expressed in human neurons. To examine whether Beclin protein is expressed in neurons (the primary CNS target cell type for Sindbis virus infection),we performed immunoperoxidase staining of adult human brain sections.We used rabbit immune serum 843, generated against a human Beclinpeptide corresponding to aa 1 to 15. 843 reacts with a 61-kDaprotein in lysates prepared from BHK cells after infection witha recombinant Sindbis virus containing a flag epitope-tagged humanbeclin insert (SIN/beclin) (Fig. 3B). This protein migrates identicallyto the major band detected with an anti-flag epitope antibodyin SIN/beclin-infected BHK cell lysates (Fig. 3A) and to in vitrotranslated flag-Beclin (data not shown). Immunoperoxidase stainingof human brain sections from the hippocampus and frontal cortexrevealed Beclin immunoreactivity in many neurons throughout theseregions as well as in some glial cells. In neurons, Beclin demonstrateda granular, punctate pattern of staining that was found almostexclusively in the region of the perikaryon (Fig. 2B). Beclinimmunoreactivity was also observed in the media of blood vessels,in the ependymal cells, and in the choroid plexus. No stainingwas observed in human brains stained with rabbit preimmune serum843 (data not shown).

View larger version (49K):
[in this window]
[in a new window]

FIG. 3. Expression of flag-Beclin protein constructs by the virus vectors SIN/beclin, SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BD. (A and B) Western blot analyses of virus-infected BHK cell lysates with either anti-flag epitope antibody M2 (A) or polyclonal rabbit anti-Beclin antiserum (B). Lane 1, SIN/beclin; lane 2, SIN/beclinstop; lane 3, SIN/beclin $Delta$ Bcl-2BD; lane 4, empty Sindbis virus vector. (C to E) Immunoperoxidase staining using anti-flag epitope antibody M2 of mouse brains 2 days after infection with SIN/beclin (C), SIN/beclinstop (D), or SIN/beclin $Delta$ Bcl-2BD (E). Magnification, ×111.

Interaction of Beclin and Bcl-2. We performed additional yeast two-hybrid studies to confirm that human beclin, like mouse beclin, encodes a protein that interactswith human Bcl-2 and to further define the Bcl-2-interacting regionof human Beclin (Table 1). We found that the region of humanBeclin that corresponds to the mouse gene product isolated inthe yeast two-hybrid screen (aa 1 to 236) also interacts withBcl-2. Further deletion mutation analysis revealed that aa 88to 150 of Beclin were sufficient to mediate an interaction withBcl-2. Interestingly, the coding sequence for this region of Beclinis deleted in some human infant brain cDNA clones in the MerckEST database, suggesting that Beclin exists in at least two forms,including one that contains a Bcl-2-binding domain and one thatlacks this domain. Full length-Beclin does not interact with Bcl-2in the yeast two-hybrid system. As noted below, when expressedin transient transfection assays, flag-tagged full-length humanBeclin displays a punctate immunoreactivity pattern suggestiveof association with intracellular organelles and is associatedwith the insoluble fraction after cell lysis. In contrast, a flag-taggedtruncated Beclin (aa 1 to 236) (corresponding to the region isolatedin the yeast two-hybrid screen) displays a diffuse cytoplasmicstaining pattern and is soluble after cell lysis. These differencesbetween full-length and truncated Beclin are thought to accountfor differences in ability to translocate to yeast nuclei andinteract with Bcl-2 in the yeast two-hybrid assay.

To directly examine whether full-length human Beclin and Bcl-2 interact in mammalian cells, we performed FRET studies of COS7cells cotransfected with Bcl-2 and flag epitope-tagged Beclin.Beclin is predicted to be a coiled-coil protein that may be associatedwith the cytoskeleton, and it partitions with the insoluble fractionfollowing cell lysis. For this technical reason, biochemical analysesof in vivo interactions between Bcl-2 and Beclin cannot be performed.FRET is a fluorescence technique that can be used as a spectroscopicruler to study and quantify the interactions of cellular componentswith each other (reviewed in references 6, 12, and 35).In FRET, a fluorophore (donor) in an excited state may transferits excitation energy to a neighboring chromophore (acceptor)nonradiatively through dipole-dipole interactions. The efficiencyof this process varies as the inverse of the sixth power of thedistance separating the donor and acceptor chromophores and, inpractice, requires the distance between the donor and acceptorfluorophores to be short (usually less than 50 Å). The dependenceof the energy transfer efficiency on the donor-acceptor separationprovides the basis for the utility of this phenomenon in the studyof cell component interactions. FRET has been used by a numberof investigators to examine interactions of cellular constituents(reviewed in 6, 12, and 35) such as endosomal fusion events,ligand-dependent growth factor receptor aggregations, interactionsof viral and cellular proteins with regulators of apoptosis (20),and interactions of cellular cytoskeletal components (33).

Prior to measuring FRET, we first confirmed the colocalization of full-length Bcl-2 and Beclin in transfected COS7 cells,using confocal laser microscopy (Fig. 4). Bcl-2 is known to associatewith the outer mitochondrial membrane, endoplasmic reticulum,and perinuclear membranes, and it displays a punctate patternof cytoplasmic immunoreactivity (reviewed in reference 28).We found that flag-Beclin invariably displayed a pattern of immunoreactivityidentical to that of Bcl-2 in all cotransfected COS7 cells examinedby confocal laser microscopic analysis (Fig. 4A to C). Furthermore,we found that deletion of the putative Bcl-2-binding domain fromBeclin did not alter its pattern of immunoreactivity; flag-Beclin $Delta$ Bcl-2BDappeared to have a pattern of staining similar to that of full-lengthBeclin, and like full-length Beclin, it colocalized with Bcl-2in cotransfected cells (Fig. 4D to F). This granular pattern ofBeclin immunoreactivity in the perinuclear region is similar tothat observed for endogenous Beclin in human neurons (compareFig. 2B, 4A, and 4D).

View larger version (79K):
[in this window]
[in a new window]

FIG. 4. Confocal laser scanning microscopy of COS7 cells expressing Bcl-2 and Beclin. (A and B) Cell cotransfected with pSG5/bcl-2 and pSG5/flag-beclin and stained with anti-flag epitope (A) and anti-human Bcl-2 (B) antibodies. (D and E) Cell cotransfected with pSG5/bcl-2 and pSG5/flag-beclinDBcl-2BD and stained with anti-flag epitope (D) and anti-human Bcl-2 (E) antibodies. (C and F) Computerized overlays of panels A and B (C) and panels D and E (F); yellow color corresponds to overlap of FITC and rhodamine staining. Confocal slides were 1 µm thick.

After confirming the colocalization of Bcl-2 and Beclin and of Bcl-2 and Beclin $Delta$ Bcl-2BD, we used FRET analysis to determinewhether Bcl-2 and Beclin physically interact. We compared in transfectedCOS7 cells the amounts of FRET between Bcl-2 and full-length Beclin,Bcl-2 and Beclin $Delta$ Bcl-2BD, and Bcl-2 and a control protein, SERCA.Quantitative analysis of microscopic images (following correctionsfor cross-talk between filter sets and donor and acceptor concentrations)showed significantly more FRET in cells with labeled full-lengthBeclin and Bcl-2 (E_Beclin-Bcl-2 = 0.000578 ± 0.000262; mean ±standard error of the mean [SEM], n = 410) than in cells withlabeled Beclin $Delta$ Bcl-2BD and Bcl-2 (E_{BeclinBcl-2BD-Bcl-2} =0.000189 ± 0.000151; n = 2,946) (P = 0.0068, t test) or in cellswith labeled SERCA and Bcl-2 (E_SERCA-Bcl-2 = 0.0000639 ± 0.0000390;n = 775) (P = 0.0021, t test). These quantitative analyses indicatethat Beclin and Bcl-2 exhibit FRET and provide evidence of aninteraction between these two proteins in mammalian cells. Furthermore,deletion of the Bcl-2-binding domain of Beclin mapped in yeasttwo-hybrid studies does not alter the spatial orientation of transfectedBeclin, but it does significantly decrease FRET. This observationsuggests that the FRET observed between full-length Beclin andBcl-2 reflects a specific association of these proteins in vivo,rather than an artifact secondary to overexpression.

Selective interaction of Beclin with death repressor members of the Bcl-2 family. To investigate whether Beclin interacts with other Bcl-2 family members that positively or negatively regulate apoptosis,we fused bax, bcl-x_S, and bcl-x_L into the GAL4 binding domainvector and tested for interactions with Beclin in the yeast two-hybridsystem (Table 1). The Bcl-x_S GAL4 binding domain construct activatedtranscription by itself and therefore could not be tested forinteractions with Beclin. The same region of Beclin (aa 88 to150) that interacted with Bcl-2 also interacted with Bcl-x_L, arelated Bcl-2 family member that inhibits apoptosis (4). Incontrast, Beclin did not react with Bax, a family member thatpromotes apoptosis (27). This pattern of interaction, i.e.,with Bcl-2 and Bcl-x_L, but not Bax, is identical to that observedfor all previously identified Bcl-2-interacting proteins outsidethe Bcl-2 family (reviewed in reference 30).

Mutations in Bcl-2 and Bcl-x_L that block death repressor activity also block binding to Beclin. Cheng et al. have shown that Bcl-2 and Bcl-x_L overexpression can delay Sindbis virus-induced death of BHK cells (5). Toevaluate whether Bcl-2-Beclin and Bcl-x_L-Beclin interactions maybe related to this ability of Bcl-2 and Bcl-x_L to inhibit Sindbisvirus-induced apoptosis, we constructed pGBT9 vectors containingbcl-2 and bcl-x_L constructs with mutations in the conserved BH1domain that are known to block death repressor activity. A Gly-Alamutation at amino acid position 145 of Bcl-2 completely abrogatesBcl-2 death repressor activity in interleukin-3 deprivation-, $gamma$ -irradiation- and glucocorticoid-induced apoptosis (42) andalso blocks Bcl-2 binding to Beclin in the yeast two-hybrid system(Table 2). Similarly, substitution of aa 136 to 138 of Bcl-x_L(VNX $right-arrow$ AIL) completely abolishes death repressor activity in Sindbisvirus-induced apoptosis (5) and also blocks Bcl-x_L bindingto Beclin (Table 2). These mutations in Bcl-2 (G $right-arrow$ A145) and Bcl-x_L(VNW $right-arrow$ AIL) did not alter the level of Bcl-2 or Bcl-x_L expressionin yeast cells (data not shown), indicating that the lack of interactioncould not be attributed to effects of the mutations on proteinexpression in yeast. These data therefore demonstrate that mutationsthat block the antideath activity of Bcl-2 and Bcl-x_L also blockbinding to Beclin.

View this table:
[in this window]
[in a new window]

TABLE 2. Effect of BH1 domain mutations on the ability of Bcl-2 and Bcl-x_L to bind to Beclin in the yeast two-hybrid assay

Beclin protects mice against fatal encephalitis caused by the neurovirulent TE12 strain of Sindbis virus. After identifying Beclin as a novel Bcl-2-interacting protein that is expressed in neurons, we were interested in studyingits effects on Sindbis virus infection. To directly evaluate therole of Beclin and its potential interactions with Bcl-2-likeproteins in modulating Sindbis virus pathogenesis, we comparedthe natural histories of mice infected with recombinant chimericviruses that express either wild-type human Beclin (SIN/beclin),human Beclin lacking the putative Bcl-2-binding domain (SIN/beclin $Delta$ Bcl-2BD),or human Beclin containing a premature stop codon at nucleotideposition 270 (SIN/beclinstop).

To construct these viruses, we used a strategy identical to that previously described for Sindbis virus chimeras that expresshuman Bcl-2 (17), with the exception that we used a more neurovirulentbackground strain of Sindbis virus, dsTE12. We chose dsTE12 ratherthan the previously used less virulent strain ds633 because ofthe possibility that the larger size of the human beclin openreading frame insert would have an attenuating effect on Sindbisvirus neurovirulence. Whereas ds633 is neurovirulent only in neonatalmice, dsTE12 is also neurovirulent in older mice (40). ds633and dsTE12 differ at one amino acid position in the E2 envelopeglycoprotein (Gln-55 in ds633; His-55 in dsTE12) and two aminoacid positions in the E1 glycoprotein (Val-72 and Gly-313 in ds633;Ala-72 and Asp-313 in dsTE12). Previous studies with recombinantviruses have mapped the amino acid residue responsible for neurovirulencein older mice to position 55 in E2 (40, 41).

We confirmed that SIN/beclin and SIN/beclin $Delta$ Bcl-2BD expressed proteins of the predicted molecular weights by performing Westernblot analyses of infected BHK cell lysates with both an anti-flagepitope monoclonal antibody and a polyclonal anti-human Beclinpeptide antibody (Fig. 3A and B). SIN/beclin expressed a 61-kDaprotein and SIN/beclin $Delta$ Bcl-2BD expressed a 52-kDa protein reactivewith both anti-flag epitope and anti-Beclin antibodies. We alsoconfirmed that human flag-Beclin and flag-Beclin $Delta$ Bcl-2BD wereexpressed in virally infected neurons by performing immunoperoxidasestaining of mouse brains at days 1, 2, and 4 after infection (representativephotomicrographs shown in Fig. 3C and E). Although we did notdetect any flag-Beclin protein expression by Western blot analysisof BHK cell lysates infected with SIN/beclinstop, flag immunoreactivitywas also observed in mouse brains infected with SIN/beclinstop(Fig. 3D). No flag immunoreactivity was seen in control mousebrains infected with the dsTE12 vector alone (data not shown).Fewer flag-immunoreactive cells were observed in SIN/beclin-infectedthan in SIN/beclin $Delta$ Bcl-2- and SIN/beclinstop-infected mouse brains.

We compared the survival of 10-day-old litters of CD1 mice infected intracerebrally with 1,000 PFU of SIN/beclin, SIN/beclin $Delta$ Bcl-2BD,and SIN/beclinstop (Fig. 5A). The survival of mice infected withSIN/beclin was 71%, compared with only 9 and 7% after infectionwith SIN/beclin $Delta$ Bcl-2BD and SIN/beclinstop. The differences insurvival between groups infected with SIN/beclin versus SIN/beclin $Delta$ Bcl-2BDand SIN/beclin versus SIN/beclinstop were highly significant (P< 0.001; life-table analysis). Thus, full-length Beclin overexpressionin virally infected neural cells results in marked protectionagainst fatal Sindbis virus encephalitis. Furthermore, the highmortality after infection with a virus expressing a mutant formof Beclin lacking the Bcl-2-binding domain suggests that bindingto Bcl-2 or Bcl-2-like proteins is important for the protectiveeffects of Beclin on survival in Sindbis virus encephalitis.

View larger version (14K):
[in this window]
[in a new window]

FIG. 5. Effects of Beclin and Bcl-2 on the survival of mice infected with Sindbis virus strain TE12. (A) Survival curve of mice infected with SIN/beclin, SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BD. Data represent combined survival probabilities for four to six independent litters. (B) Survival curve of mice infected with SIN/bcl-2 and SIN/bcl-2stop. Data represent combined survival probabilities for three independent litters.

Bcl-2 does not protect against fatal encephalitis caused by TE12. Previously, we showed that Bcl-2, expressed in the ds633 Sindbis virus vector, protected neonatal mice against fatal Sindbisvirus infection (17). However, in in vitro studies in AT3/bcl-2cells, the TE12 strain overcomes protection conferred by Bcl-2(41). To directly compare the abilities of Beclin and Bcl-2to protect against encephalitis by TE12 in 10-day-old mice, wecloned human bcl-2 and human bcl-2 containing a premature stopcodon after nucleotide position 118 into the dsTE12 vector togenerate the constructs SIN/bcl-2 and SIN/bcl-2stop. Unlike SIN/beclinversus SIN/beclinstop (Fig. 5A), there was no difference in thesurvival of mice infected with SIN/bcl-2 versus SIN/bcl-2stop(Fig. 5B). Together with previous results (17), these data demonstratethat Bcl-2 can protect against fatal encephalitis caused by astrain of Sindbis virus containing a wild-type glutamine at positionE2 position 55 but not by a more neurovirulent strain of Sindbisvirus containing a histidine mutation at E2 position 55 (E2-55histidine mutation).

Beclin reduces Sindbis virus replication in mouse brain. To examine whether Beclin overexpression affects Sindbis virus replication, we measured viral titers of mouse brain homogenatesand performed in situ hybridization of mouse brain sections todetect message-sense viral RNA. Mean viral titers were reduced5-fold at day 1 and 50-fold at days 2 and 4 after infection inbrains of mice infected with SIN/beclin compared to the brainsof mice infected with SIN/beclinstop or SIN/beclin $Delta$ bcl-2BD (Fig.6). Computerized quantitative image analysis of virus RNA positivecells in infected mouse brains showed an inhibitory effect ofBeclin on viral replication that was similar to, but had a temporalpattern somewhat different from, that observed by measurementof viral titers (Fig. 7). The mean number of virus RNA-positivecells was significantly lower in brains infected with SIN/beclinthan in brains infected with SIN/beclinstop at day 4 after infection(100 ± 36 versus 494 ± 55; P = 0.004, t test) but was equivalentat day 2 after infection (575 ± 272 versus 507 ± 216; P = 0.854,t test). The reduction of viral titers but not of virus RNA-positivecells in mouse brains 2 days after infection with SIN/beclin suggestsa possible inhibitory effect of Beclin on posttranscriptionalstages of viral replication. In addition, the viral titers ofSIN/beclin $Delta$ Bcl-2BD-infected mouse brains did not differ significantlyfrom titers of SIN/beclinstop-infected mouse brains, but the numberof virus RNA-positive cells was higher at days 2 and 4 in SIN/beclin $Delta$ Bcl-2BD-infected than in SIN/beclinstop-infected mousebrains. This difference was significant at day 4 (905 ± 72 versus494 ± 55; P = 0.01, t test) but not at day 2 (1,190 ± 375 versus507 ± 216; P = 0.190, t test) after infection.

View larger version (15K):
[in this window]
[in a new window]

FIG. 6. Viral growth of SIN/beclin, SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BD in mouse brain. Each data point represents geometric mean viral titer ± SEM of three to six mouse brains.

View larger version (18K):
[in this window]
[in a new window]

FIG. 7. Viral RNA-positive cells in mouse brains infected with SIN/beclin, SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BD. Each data point represents the mean ± SEM number of Sindbis virus message-sense RNA-positive cells per square millimeter of brain for three to six mouse brains.

The anatomic distribution of RNA-positive cells did not differ among the different virus-infected groups; viral RNA-positivecells were found in clusters scattered throughout the brain, mostcommonly in the subventricular zone, posterior neocortex, colliculus,hippocampus, striatum, and olfactory bulb. However, the numberof cells seen within a given cluster was usually lowest in SIN/beclin-infectedmouse brains and greatest in SIN/beclin $Delta$ Bcl-2BD-infected mousebrains (see representative photomicrographs in Fig. 9).

Beclin reduces Sindbis virus-induced cell death in mouse brain. To examine whether CNS Beclin overexpression reduces apoptotic cell death, we quantitated the number of apoptotic nuclei inthe brains of mice infected with the chimeric viruses SIN/beclin,SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BD (Fig. 8). Within each mousebrain, almost all apoptotic nuclei were found in regions thathad detectable viral RNA by in situ hybridization (Fig. 9) andin regions that had histopathologic evidence of neuronal death.A close association was observed between the mean numbers of apoptoticnuclei at each time point among the three different virus treatmentgroups and the mean numbers of virus RNA-positive cells (compareresults in Fig. 7 and 8). In mouse brains infected with SIN/beclinand SIN/beclinstop, little cell death was seen at days 1 and 2after infection, and the number of apoptotic cells per squaremillimeter of brain did not differ between these groups. Moreapoptotic nuclei were present at day 2 after infection in thebrains of mice infected with SIN/beclin $Delta$ Bcl-2BD (604 ± 211) thanin the brains of mice infected with SIN/beclin (133 ± 90) or SIN/beclinstop(91 ± 52); this difference was nearly statistically significant(P = 0.078, analysis of variance). At day 4 after infection, themean number of apoptotic cells per square millimeter of brainwas markedly increased in SIN/beclinstop (1,490 ± 29) and SIN/beclin $Delta$ Bcl-2BD(1,044 ± 430) versus SIN/beclin-infected mouse brains (101 ± 10;P = 0.001, analysis of variance). These data demonstrate thatBeclin overexpression decreases apoptotic death in mouse brainsinfected with the TE12 strain of Sindbis virus.

View larger version (20K):
[in this window]
[in a new window]

FIG. 8. Apoptotic nuclei in mouse brains infected with SIN/beclin, SIN/beclinstop, and SIN/beclin $Delta$ Bcl-2BD. Each data point represents the mean ± SEM number of ISEL-positive nuclei per square millimeter of brain for three to six mouse brains.

View larger version (71K):
[in this window]
[in a new window]

FIG. 9. Representative photomicrographs of fields used for computerized quantitative image analysis of viral RNA (A to C)- and ISEL (D to F)-positive cells in mouse brains infected with SIN/beclin (A and D), SIN/beclinstop (B and E), and SIN/beclin $Delta$ Bcl-2BD (C and F) in Fig. 7 and 8, respectively. All photomicrographs are from the colliculus region of brain sections 4 days after infection and correspond to the images observed at a magnification of ×10. Arrowheads denote representative cells that were scored as positive by the Image-ProPlus software program.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this study, we describe the identification of a novel coiled-coil 60-kDa protein, Beclin, which interacts with the celldeath regulator Bcl-2. We demonstrate that Beclin overexpressionin virally infected neurons in vivo results in substantial protectionagainst Sindbis virus-induced disease. Mice infected with recombinantSindbis viruses that express wild-type Beclin have less neuralcell apoptosis, decreased viral replication, and a significantlower mortality rate than mice infected with recombinant virusesthat express Beclin deletion mutants. Furthermore, the Bcl-2-bindingdomain of Beclin is required for the antiviral, antiapoptotic,and survival-promoting effects of Beclin on CNS Sindbis virusinfection. These findings suggest that Beclin, via interactionswith Bcl-2-like molecules, can function in vivo in the CNS asan antiviral host defense molecule.

Our conclusion that the protective, antiviral effects of Beclin are mediated through interactions with Bcl-2 (or Bcl-2-likemolecules that bind to same region of Beclin as Bcl-2) is supportedby data obtained with a chimeric Sindbis virus expressing Beclinlacking aa 88 to 151. Amino acids 88 to 150 of Beclin are sufficientto mediate an interaction with Bcl-2 and Bcl-x_L in the yeast two-hybridassay, and deletion of these amino acids from full-length Beclinsignificantly decreases the strength of the Beclin-Bcl-2 interactionin mammalian cells. The Sindbis virus construct expressing Beclinlacking aa 88 to 150 (SIN/beclin $Delta$ Bcl-2BD) replicated to as highlevels in mouse brain, resulted in as much apoptotic neural celldeath, and resulted in the same mortality in mice as a controlrecombinant virus which expressed a 90-aa truncated Beclin protein(SIN/beclinstop). The lack of protective activity of Beclin $Delta$ Bcl-2BDcompared to full-length Beclin cannot be attributed to lower levelsof Beclin $Delta$ Bcl-2BD expression after infection with SIN/beclin $Delta$ Bcl-2BD.The levels of flag-Beclin $Delta$ Bcl-2BD were equal to or greater thanlevels of flag-Beclin detected by immunoblot analysis of lysatesfrom BHK cells infected with SIN/beclin and SIN/beclin $Delta$ Bcl-2BD,respectively. In addition, SIN/beclin $Delta$ Bcl-2BD-infected mouse brainshad more flag-immunoreactive cells than mouse brains infectedwith SIN/beclin. Thus, the lack of protective activity of Beclin $Delta$ Bcl-2is most consistent with the hypothesis that the antiviral effectsof Beclin are mediated through interactions with Bcl-2-like proteins.

Some of the data in the present study suggest that the virus SIN/beclin $Delta$ Bcl-2BD may be more neurovirulent than the virus SIN/beclinstop.Mice infected with SIN/beclin $Delta$ Bcl-2BD had more virus RNA-positivecells in their brains at days 2 and 4 after infection than miceinfected with SIN/beclinstop. Corresponding to the more rapidspread of infection, more cell death was seen earlier on afterinfection in the brains of mice infected with SIN/beclin $Delta$ Bcl-2BDcompared to SIN/beclinstop. Although the overall mortality ratesof mice infected with SIN/beclin $Delta$ Bcl-2BD versus SIN/beclin stopdid not differ, but the mean day of death was slightly lower inmice infected with SIN/beclin $Delta$ Bcl-2BD versus SIN/beclinstop. Theseobservations raise the possibility that Beclin lacking the Bcl-2-bindingdomain functions as a dominant negative mutant. As a corollary,the naturally occurring Beclin isoform found in brain that lacksthe Bcl-2-binding domain may serve as a death-promoting molecule.

Beclin may exert antiviral effects via interactions with either Bcl-2, Bcl-x_L, or yet unidentified Bcl-2 family members. Inyeast two-hybrid assays, we found that the same region of Beclininteracted with Bcl-2 and Bcl-x_L and that loss-of-function mutationsin the conserved BH1 domains of both Bcl-2 and Bcl-x_L blockedbinding to Beclin. While both Bcl-2 and Bcl-x_L are important regulatorsof apoptosis in neurons (reviewed in reference 23), we havefound that Bcl-2, but not Bcl-x_L, protects mice against fatalencephalitis and delays Sindbis virus-induced death of culturedrat dorsal root ganglion neurons (14, 17). Thus, Bcl-2 maybe more important than Bcl-x_L as a regulator of Sindbis virus-induceddeath in neural cells. Additional studies examining the effectsof Beclin on Sindbis virus infection in mice that are deficientin Bcl-2 may help define whether Bcl-2 is the biologically importantBeclin-binding partner in in vivo antiviral pathways in the CNS.

The mechanisms by which Beclin, in cooperation with Bcl-2-like proteins, functions to inhibit Sindbis virus replication andSindbis virus-induced neuronal death are unknown. Both SemlikiForest virus and Sindbis virus have been shown to inactivate theantiapoptotic function of Bcl-2 in transfected fibroblasts throughcaspase-induced Bcl-2 cleavage (10). In addition, Nava et al.have shown that crmA increases the survival of Sindbis virus-infectedmice (24), suggesting a role for crmA-inhibitable CNS caspaseactivity in the pathogenesis of fatal encephalitis. One possibility,therefore, is that binding to Beclin somehow protects Bcl-2 (orBcl-x_L) from cleavage by caspases, thereby preventing Sindbisvirus-induced cell death. A second possibility is that the Beclin-Bcl-2-likeprotein complex blocks an endoplasmic reticulum stress signaltriggered by the Sindbis virus E2 and E1 envelope glycoproteins.One of the mechanisms by which Bcl-2 and Bcl-may inhibit apoptosisis by regulating the permeability of intracellular membranes (reviewedin reference 30). Recently, we have shown that the overexpressionof the transmembrane domains of the Sindbis virus E2 and E1 envelopeglycoproteins induces apoptosis in AT3 cells (15). In addition,coiled-coil proteins such as Beclin may play a role in linkingmembrane signal transduction events with the cytoskeleton. Thus,we speculate that Beclin, a protein which localizes to intracellularmembranes, may be part of a complex with Bcl-2-like proteins thatregulates signalling events initiated by Sindbis virus envelopeglycoproteins in the endoplasmic reticulum.

Many similarities exist between the findings of the present study and our previous work examining the effects of Bcl-2 overexpressionon the natural history of Sindbis virus encephalitis. As observedwith Beclin in this study, the overexpression of Bcl-2 in virallyinfected neurons has previously been shown to reduce CNS apoptosis,reduce CNS Sindbis virus replication, and reduce Sindbis virusmortality (17). However, in the present study, we also identifyone significant biologic difference between Bcl-2 and Beclin;namely, Beclin can exert protective effects against infectionby a neurovirulent strain of Sindbis virus that is known to overcomethe protective effects of Bcl-2. Ubol et al. demonstrated thata histidine substitution for wild-type glutamine at position 55of the Sindbis virus E2 envelope glycoprotein was sufficient toenable the virus to kill cells expressing Bcl-2 (41). Similarly,we have previously found that Bcl-2 expressed in a strain of Sindbiscontaining a glutamine at position 55 (strain 633) protects againstfatal encephalitis (17), but in the present study, we foundthat Bcl-2 expressed in a strain of Sindbis containing a histidineat position 55 (strain TE12) confers no protection against fataldisease. Yet, when expressed in an E2-55 histidine-containingbackground strain of Sindbis virus, Beclin confers significantprotection. Thus, the mutation in E2, which confers neurovirulence,can counter the protective effects of Bcl-2 but not of Beclin.

Several explanations have been proposed to explain the ability of the E2-55 histidine mutation to confer resistance to Bcl-2protection against Sindbis virus-induced death. Ubol et al. suggestedthat the neurovirulent mutation in E2 might somehow alter eithera direct interaction between E2 and Bcl-2 in the endoplasmic reticulumor a possible effect of Bcl-2 on E2 protein folding or posttranslationalmodifications (41). More recently, Grandgirard et al. raisedthe possibility that the mutation in E2 facilitates the accessof caspases to Bcl-2 and subsequent triggering of Bcl-2 cleavage(10). If viral activation of caspase-induced cleavage of Bcl-2does prove to be an important mechanism of neurovirulence of Sindbisvirus strains containing E2-55 histidine, our data suggest thatBeclin may serve as an important host defense factor against thisstrategy of neurovirulence. This hypothesis is based on the abilityof Beclin, a Bcl-2-interacting protein, to protect against neuronaldeath induced by the TE12 strain of Sindbis virus.

Our findings suggest that the antiviral effects of Beclin observed in Sindbis virus-infected mouse brains may be exerted ata stage of viral replication after viral RNA synthesis. At 2 daysafter chimeric virus infection, Beclin overexpression was associatedwith a 50-fold reduction in viral titers but no reduction in thenumber of viral RNA-positive cells. This finding suggests a blockor abnormality at the level of either translation of the Sindbisvirus structural proteins, posttranslational modifications ofviral glycoproteins, virus assembly, or budding. This observationcontrasts with previous studies examining the effects of Bcl-2on infection with a related alphavirus, Semliki Forest virus (34).On the basis of in situ hybridization studies for viral RNA andimmunostaining for viral proteins, Scallan et al. concluded thatbcl-2 functions at an early stage of the virus life cycle, eitherentry, pretranscriptional events, or transcription, to inhibitSemliki Forest virus replication (34). The discrepancy betweenthe findings of Scallan et al. and those reported in the presentstudy may reflect fundamental differences between the antiviraleffects of Beclin and Bcl-2, differences between Sindbis virusand Semliki Forest virus, or differences between the cell typesinfected. Alternatively, it is possible that Bcl-2 and/or Beclinact at multiple overlapping stages of the alphavirus life cycleand that different experimental designs in the two studies uncoveredeffects on different phases of replication. Given the lack ofantiviral activity of Beclin lacking the Bcl-2-binding domain,it seems likely that the mechanisms by which Beclin and Bcl-2inhibit Sindbis virus replication in mouse brain are similar.

The results of the present study do not permit us to evaluate whether the beneficial effects of Beclin on Sindbis virus-inducedmortality are a consequence of antiviral effects, antiapoptoticeffects, or a combination of both. It is not known whether Beclinprevents neural cell death solely as a consequence of reducingSindbis virus replication in neurons or whether Beclin exertsantiapoptotic effects independently of its effects on viral replication.Further studies examining the effects of Beclin on apoptotic deathin response to nonviral stimuli will be necessary to determinewhether Beclin, like Bcl-2, functions as a general apoptosis inhibitor.If so, structure-function analyses of Beclin may be helpful tomap domains important for antiviral and antiapoptotic functionand to identify whether these two properties are interrelatedor independent.

Previously, based on our observations with Bcl-2 and Sindbis virus infection, we postulated that molecular links may existbetween cellular regulation of viral replication and cellularregulation of apoptotic death in neurons (17). Our findingsthat Beclin has antiviral activity and that Beclin interacts withthe cell death regulator Bcl-2 further support this hypothesis.In dividing cells, inhibition of virus-induced cell death by virallyencoded cell death inhibitors such as p35 (7) and adenovirusE1B can increase viral replication (3). However, in nondividing,terminally differentiated cells such as neurons, genetic pathwaysmay exist which permit preservation of the life of the cell, withoutthe adverse consequence of increased total viral burden for theorganism. Genes such as bcl-2 and beclin that are normally expressedin mammalian neurons may be important components of such pathways.

	ACKNOWLEDGMENTS

The first two authors contributed equally to this work.

We thank M. B. Soares for providing the normalized human infant brain cDNA library, Takaki Sato for providing bcl-x_S, bcl-x_L,and bax plasmids, Steven Greenberg and Milton Packer for helpfuldiscussions, and Tracey Curran for secretarial assistance.

This work was supported by a James S. McDonnell Foundation Scholar Award (B.L.) and NIH grants AIO1217 (B.L.), AI40246 (B.L.),AG07218 (B.H.), AG13797 (B.H.), and AG13637 (B.H.). B.L. was supportedby an American Cancer Society Junior Faculty Research Award andan Irma T. Hirschl Trust Career Scientist Award.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Medicine, Columbia University College of Physicians and Surgeons, 630W. 168th St. P & S 8-444, New York, NY 10032. Phone: (212) 305-7312.Fax: (212) 305-7290. E-mail: Levine{at}cuccfa.ccc.columbia.edu.

Present address: Department of Cellular and Structural Biology, University of Texas Health Science Center at San Antonio,San Antonio, TX 78284.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Allsopp, T. E., M. F. Scallan, A. Williams, and J. K. Fazakerley. 1998. Virus infection induces neuronal apoptosis: a comparison with trophic factor withdrawal. Cell Death Differ. 5:50-59. [Medline]

2. Altshul, S. F., W. Gish, W. Miller, E. W. Meyers, and D. J. Lipman. 1990. Basic local alignment tool. J. Mol. Biol. 215:403-410[Medline].

3. Antoni, B. A., P. A. Sabbatini, A. B. Rabson, and E. White. 1995. Inhibition of apoptosis in human immunodeficiency virus-infected cells enhances virus production and facilitates persistent infection. J. Virol. 69:2384-2392[Abstract].

4. Boise, L. H., M. Gonzalez-Garcia, C. E. Postema, L. Ding, T. Lindsten, L. A. Turka, X. Mao, G. Nunez, and C. B. Thompson. 1993. Bcl-x_L, a bcl-2 related gene that functions as a dominant regulator of apoptotic cell death. Cell 74:597-608[Medline].

5. Cheng, E. H. Y., B. Levine, L. H. Boise, C. B. Thompson, and J. M. Hardwick. 1996. Bax-independent inhibition of apoptosis by Bcl-x_L. Nature 379:554-556[Medline].

6. Clegg, R. M. 1992. Fluorescence resonance energy transfer and nucleic acids. Methods Enzymol. 211:353-388[Medline].

7. Clem, R., and L. K. Miller. 1993. Apoptosis reduces both the in vitro replication and the in vivo infectivity of baculovirus. J. Virol. 67:3730-3738[Abstract/Free Full Text].

8. Friedman, L. S., E. A. Ostermeyer, E. D. Lynch, C. I. Szabo, L. A. Anderson, P. Dowd, M. K. Lee, S. E. Rowell, J. M. Boyd, and M.-C. King. 1994. The search for BRCA1. Cancer Res. 54:6374-6382[Abstract/Free Full Text].

9. Gordon, G. W., G.- Berry, X. H. Liang, B. Levine, and B. Herman. 1998. Quantitative fluorescence resonance energy transfer (FRET) measurements using fluorescence microscopy. Biophys. J. 74:2702-2713[Abstract/Free Full Text].

10. Grandgirard, D., E. Studer, L. Monney, T. Belser, I. Fellay, C. Borner, and M. R. Michel. 1998. Alphaviruses induce apoptosis in Bcl-2-overexpressing cells: evidence for a caspase-mediated, proteolytic inactivation of Bcl-2. EMBO J. 17:1268-1278[Medline].

11. Hardwick, J. M. 1997. Virus-induced apoptosis. Adv. Pharmacol. 41:295-336.

12. Herman, B. 1996. Fluorescence microscopy: state of the art, p. 1-14. In J. Slavik (ed.), Fluorescent microscopy and fluorescent probes. Plenum Press, New York, N.Y.

13. Hinshaw, V. S., C. W. Olsen, N. Dybdahl-Sissoko, and D. Evans. 1994. Apoptosis: a mechanism of cell killing by influenza A and B viruses. J. Virol. 68:3667-3673[Abstract/Free Full Text].

14. Jiang, H. H., and B. Levine. Unpublished data.

15. Joe, A. K., H. H. Foo, L. Kleeman, and B. Levine. 1998. The transmembrane domains of Sindbis virus envelope glycoproteins induce cell death. J. Virol. 72:3935-3943[Abstract/Free Full Text].

16. Krakauer, D. C., and R. J. Payne. 1997. The evolution of virus-induced apoptosis. Proc. R. Soc. Lond. Ser. B 264:1757-1762[Medline].

17. Levine, B., J. E. Goldman, H. H. Jiang, D. E. Griffin, and J. M. Hardwick. 1996. Bcl-2 protects mice against fatal alphavirus encephalitis. Proc. Natl. Acad. Sci. USA 93:4810-4815[Abstract/Free Full Text].

18. Levine, B., Q. Huang, J. T. Isaacs, J. C. Reed, D. E. Griffin, and J. M. Hardwick. 1993. Conversion of lytic to persistent alphavirus infection by the bcl-2 cellular oncogene. Nature 361:739-742[Medline].

19. Lewis, J., S. L. Wesslingh, D. E. Griffin, and J. M. Hardwick. 1996. Alphavirus-induced apoptosis in mouse brains correlates with neurovirulence. J. Virol. 70:1828-1835[Abstract].

20. Liang, X. H., M. Volkmann, R. Klein, B. Herman, and B. Lockett. 1994. Colocalization of tumor suppressor protein p53 and human papillomavirus E6 protein in human cervical carcinoma cell lines. Oncogene 8:2645-2652.

21. Liao, C. L., Y. L. Lin, J. J. Wang, Y. L. Huang, C. T. Yeh, S. H. Ma, and L. K. Chen. 1997. Effect of enforced expression of human bcl-2 on Japanese encephalitis virus-induced apoptosis in cultured cells. J. Virol. 71:5963-5971[Abstract].

22. Lupas, A., M. Van Dyke, and M. J. Stock. 1991. Predicting coiled coils from protein sequences. Science 252:1162-1164[Medline].

23. Merry, D. E., and S. J. Korsmeyer. 1997. Bcl-2 gene family in the nervous system. Annu. Rev. Neurosci. 20:245-267[Medline].

24. Nava, V. E., A. Rosen, M. A. Veliuona, R. J. Clem, B. Levine, and J. M. Hardwick. 1998. Sindbis virus induces apoptosis through a caspase-dependent CrmA-sensitive pathway. J. Virol. 72:452-459[Abstract/Free Full Text].

25. Oberhaus, S. M., R. L. Smith, G. W. Clayton, T. S. Dermody, and K. L. Tyler. 1997. Reovirus infection and tissue injury in the mouse central nervous system are associated with apoptosis. J. Virol. 71:2100-2106[Abstract].

26. Olsen, C. W., J. C. Kehren, N. R. Dybdahl-Sissoki, and V. S. Hinshaw. 1996. bcl-2 alters influenza virus, yield, spread, and hemagglutinin glycosylation. J. Virol. 80:663-666.

27. Oltvai, Z., C. L. Milliman, and S. J. Korsmeyer. 1993. Bcl-2 heterodimerizes in vivo with a conserved homolog, Bax, that accelerates programmed cell death. Cell 74:609-619[Medline].

28. Park, J. R., and D. M. Hockenbery. 1996. Bcl-2, a novel regulator of apoptosis. J. Cell. Biochem. 60:12-17[Medline].

29. Pekosz, A., J. Phillips, D. Pleasure, D. Merry, and F. Gonzalez-Scarano. 1996. Induction of apoptosis by LaCrosse virus infection and role of neuronal differentiation and human bcl-2 expression in its prevention. J. Virol. 70:5329-5335[Abstract/Free Full Text].

30. Reed, J. C. 1997. Double identity for proteins of the Bcl-2 family. Nature. 387:773-776[Medline].

31. Rodgers, S. E., E. S. Barton, S. M. Oberhaus, B. Pike, C. A. G. Terence, K. L. Tyler, and T. S. Dermody. 1997. Reovirus-induced apoptosis of MDCK cells is not linked to viral yield and is blocked by Bcl-2. J. Virol. 71:2540-2546[Abstract].

32. Rommens, J. M., F. Durocher, J. McArthur, P. Tonin, J.-F. LeBlanc, T. Allen, C. Samson, L. Ferri, S. Narod, K. Morgan, and J. Simard. 1995. Generation of a transcription map at the HSD17B locus centromeric to BRCA1 at 17q21. Genomics 28:530-542[Medline].

33. Root, D. D. 1997. In situ molecular association of dystrophin with actin revealed by sensitized emission immuno-resonance energy transfer. Proc. Natl. Acad. Sci. USA 94:5685-5690[Abstract/Free Full Text].

34. Scallan, M. F., T. E. Allsopp, and J. K. Fazakerley. 1997. bcl-2 acts early to restrict Semliki Forest virus replication and delays virus-induced programmed cell death. J. Virol. 71:1583-1590[Abstract].

35. Selvin, P. R. 1995. Fluorescence resonance energy transfer. Methods Enzymol. 246:300-333[Medline].

36. Shen, Y., and T. E. Shenk. 1995. Viruses and apoptosis. Curr. Opin. Genet. Dev. 5:105-111[Medline].

37. Soares, M. B., M. F. Bonaldo, P. Jelene, L. Su, L. Lawton, and A. Efstradiadis. 1994. Construction and characterization of a normalized cDNA library. Proc. Natl. Acad. Sci. USA 91:9228-9232[Abstract/Free Full Text].

38. Tangir, J., M. G. Muto, R. S. Berkowitz, W. R. Welch, D. A. Bell, and S. C. Mok.

1.	Allsopp, T. E., M. F. Scallan, A. Williams, and J. K. Fazakerley. 1998. Virus infection induces neuronal apoptosis: a comparison with trophic factor withdrawal. Cell Death Differ. 5:50-59. [Medline]
2.	Altshul, S. F., W. Gish, W. Miller, E. W. Meyers, and D. J. Lipman. 1990. Basic local alignment tool. J. Mol. Biol. 215:403-410[Medline].
3.	Antoni, B. A., P. A. Sabbatini, A. B. Rabson, and E. White. 1995. Inhibition of apoptosis in human immunodeficiency virus-infected cells enhances virus production and facilitates persistent infection. J. Virol. 69:2384-2392[Abstract].
4.	Boise, L. H., M. Gonzalez-Garcia, C. E. Postema, L. Ding, T. Lindsten, L. A. Turka, X. Mao, G. Nunez, and C. B. Thompson. 1993. Bcl-x_L, a bcl-2 related gene that functions as a dominant regulator of apoptotic cell death. Cell 74:597-608[Medline].
5.	Cheng, E. H. Y., B. Levine, L. H. Boise, C. B. Thompson, and J. M. Hardwick. 1996. Bax-independent inhibition of apoptosis by Bcl-x_L. Nature 379:554-556[Medline].
6.	Clegg, R. M. 1992. Fluorescence resonance energy transfer and nucleic acids. Methods Enzymol. 211:353-388[Medline].
7.	Clem, R., and L. K. Miller. 1993. Apoptosis reduces both the in vitro replication and the in vivo infectivity of baculovirus. J. Virol. 67:3730-3738[Abstract/Free Full Text].
8.	Friedman, L. S., E. A. Ostermeyer, E. D. Lynch, C. I. Szabo, L. A. Anderson, P. Dowd, M. K. Lee, S. E. Rowell, J. M. Boyd, and M.-C. King. 1994. The search for BRCA1. Cancer Res. 54:6374-6382[Abstract/Free Full Text].
9.	Gordon, G. W., G.- Berry, X. H. Liang, B. Levine, and B. Herman. 1998. Quantitative fluorescence resonance energy transfer (FRET) measurements using fluorescence microscopy. Biophys. J. 74:2702-2713[Abstract/Free Full Text].
10.	Grandgirard, D., E. Studer, L. Monney, T. Belser, I. Fellay, C. Borner, and M. R. Michel. 1998. Alphaviruses induce apoptosis in Bcl-2-overexpressing cells: evidence for a caspase-mediated, proteolytic inactivation of Bcl-2. EMBO J. 17:1268-1278[Medline].
11.	Hardwick, J. M. 1997. Virus-induced apoptosis. Adv. Pharmacol. 41:295-336.
12.	Herman, B. 1996. Fluorescence microscopy: state of the art, p. 1-14. In J. Slavik (ed.), Fluorescent microscopy and fluorescent probes. Plenum Press, New York, N.Y.
13.	Hinshaw, V. S., C. W. Olsen, N. Dybdahl-Sissoko, and D. Evans. 1994. Apoptosis: a mechanism of cell killing by influenza A and B viruses. J. Virol. 68:3667-3673[Abstract/Free Full Text].
14.	Jiang, H. H., and B. Levine. Unpublished data.
15.	Joe, A. K., H. H. Foo, L. Kleeman, and B. Levine. 1998. The transmembrane domains of Sindbis virus envelope glycoproteins induce cell death. J. Virol. 72:3935-3943[Abstract/Free Full Text].
16.	Krakauer, D. C., and R. J. Payne. 1997. The evolution of virus-induced apoptosis. Proc. R. Soc. Lond. Ser. B 264:1757-1762[Medline].
17.	Levine, B., J. E. Goldman, H. H. Jiang, D. E. Griffin, and J. M. Hardwick. 1996. Bcl-2 protects mice against fatal alphavirus encephalitis. Proc. Natl. Acad. Sci. USA 93:4810-4815[Abstract/Free Full Text].
18.	Levine, B., Q. Huang, J. T. Isaacs, J. C. Reed, D. E. Griffin, and J. M. Hardwick. 1993. Conversion of lytic to persistent alphavirus infection by the bcl-2 cellular oncogene. Nature 361:739-742[Medline].
19.	Lewis, J., S. L. Wesslingh, D. E. Griffin, and J. M. Hardwick. 1996. Alphavirus-induced apoptosis in mouse brains correlates with neurovirulence. J. Virol. 70:1828-1835[Abstract].
20.	Liang, X. H., M. Volkmann, R. Klein, B. Herman, and B. Lockett. 1994. Colocalization of tumor suppressor protein p53 and human papillomavirus E6 protein in human cervical carcinoma cell lines. Oncogene 8:2645-2652.
21.	Liao, C. L., Y. L. Lin, J. J. Wang, Y. L. Huang, C. T. Yeh, S. H. Ma, and L. K. Chen. 1997. Effect of enforced expression of human bcl-2 on Japanese encephalitis virus-induced apoptosis in cultured cells. J. Virol. 71:5963-5971[Abstract].
22.	Lupas, A., M. Van Dyke, and M. J. Stock. 1991. Predicting coiled coils from protein sequences. Science 252:1162-1164[Medline].
23.	Merry, D. E., and S. J. Korsmeyer. 1997. Bcl-2 gene family in the nervous system. Annu. Rev. Neurosci. 20:245-267[Medline].
24.	Nava, V. E., A. Rosen, M. A. Veliuona, R. J. Clem, B. Levine, and J. M. Hardwick. 1998. Sindbis virus induces apoptosis through a caspase-dependent CrmA-sensitive pathway. J. Virol. 72:452-459[Abstract/Free Full Text].
25.	Oberhaus, S. M., R. L. Smith, G. W. Clayton, T. S. Dermody, and K. L. Tyler. 1997. Reovirus infection and tissue injury in the mouse central nervous system are associated with apoptosis. J. Virol. 71:2100-2106[Abstract].
26.	Olsen, C. W., J. C. Kehren, N. R. Dybdahl-Sissoki, and V. S. Hinshaw. 1996. bcl-2 alters influenza virus, yield, spread, and hemagglutinin glycosylation. J. Virol. 80:663-666.
27.	Oltvai, Z., C. L. Milliman, and S. J. Korsmeyer. 1993. Bcl-2 heterodimerizes in vivo with a conserved homolog, Bax, that accelerates programmed cell death. Cell 74:609-619[Medline].
28.	Park, J. R., and D. M. Hockenbery. 1996. Bcl-2, a novel regulator of apoptosis. J. Cell. Biochem. 60:12-17[Medline].
29.	Pekosz, A., J. Phillips, D. Pleasure, D. Merry, and F. Gonzalez-Scarano. 1996. Induction of apoptosis by LaCrosse virus infection and role of neuronal differentiation and human bcl-2 expression in its prevention. J. Virol. 70:5329-5335[Abstract/Free Full Text].
30.	Reed, J. C. 1997. Double identity for proteins of the Bcl-2 family. Nature. 387:773-776[Medline].
31.	Rodgers, S. E., E. S. Barton, S. M. Oberhaus, B. Pike, C. A. G. Terence, K. L. Tyler, and T. S. Dermody. 1997. Reovirus-induced apoptosis of MDCK cells is not linked to viral yield and is blocked by Bcl-2. J. Virol. 71:2540-2546[Abstract].
32.	Rommens, J. M., F. Durocher, J. McArthur, P. Tonin, J.-F. LeBlanc, T. Allen, C. Samson, L. Ferri, S. Narod, K. Morgan, and J. Simard. 1995. Generation of a transcription map at the HSD17B locus centromeric to BRCA1 at 17q21. Genomics 28:530-542[Medline].
33.	Root, D. D. 1997. In situ molecular association of dystrophin with actin revealed by sensitized emission immuno-resonance energy transfer. Proc. Natl. Acad. Sci. USA 94:5685-5690[Abstract/Free Full Text].
34.	Scallan, M. F., T. E. Allsopp, and J. K. Fazakerley. 1997. bcl-2 acts early to restrict Semliki Forest virus replication and delays virus-induced programmed cell death. J. Virol. 71:1583-1590[Abstract].
35.	Selvin, P. R. 1995. Fluorescence resonance energy transfer. Methods Enzymol. 246:300-333[Medline].
36.	Shen, Y., and T. E. Shenk. 1995. Viruses and apoptosis. Curr. Opin. Genet. Dev. 5:105-111[Medline].
37.	Soares, M. B., M. F. Bonaldo, P. Jelene, L. Su, L. Lawton, and A. Efstradiadis. 1994. Construction and characterization of a normalized cDNA library. Proc. Natl. Acad. Sci. USA 91:9228-9232[Abstract/Free Full Text].
38.	Tangir, J., M. G. Muto, R. S. Berkowitz, W. R. Welch, D. A. Bell, and S. C. Mok.