Selective Neuronal Expression of Green Fluorescent Protein with Cytomegalovirus Promoter Reveals Entire Neuronal Arbor in Transgenic Mice

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The Journal of Neuroscience, December 15, 1998, 18(24):10640-10651

Selective Neuronal Expression of Green Fluorescent Protein with Cytomegalovirus Promoter Reveals Entire Neuronal Arbor in Transgenic Mice
Anthony N. van den Pol and Prabhat K. Ghosh
Department of Neurosurgery, Yale University School of Medicine, New Haven, Connecticut 06520

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In simple nervous systems, identified groups of neurons can be studied in depth. To allow the same advantage in the mammalianbrain, we have generated green fluorescent protein (GFP) transgenicmice in which only a few types of neurons are strongly labeledwith a fluorescent molecule, which the neurons synthesize internally,allowing the cells, their dendrites, filopodia, and axons to beidentified in both living and fixed CNS, in slices and culture.The same neurons, with GFP expression controlled by part of themajor immediate early promoter of human cytomegalovirus (CMV),show GFP beginning early in development, from one generation tothe next, allowing cellular and physiological studies of axonaland dendritic growth, fate mapping, anatomical connections, andsynapse formation in identified neurons. The human CMV promotersequence we used was different from that used in previous workwith other reporter genes and gave a dramatically different patternof expression. Two transgenic lines with the same CMV promotershow similar anatomical patterns of expression in the presentstudy. Strong GFP labeling was found in a subpopulation of mossyfibers that innervated parasagittal bands in the cerebellar cortexand olfactory axons that projected into the olfactory bulb, subsetsof motoneurons and dorsal root ganglion cells, granule but notmitral cells of the olfactory bulb, and a group of neurons inthe hypothalamic suprachiasmatic nucleus. A novel type of neuronwas strongly labeled in the olfactory bulb external plexiformlayer. In normal brains, CMV does not constitute a threat, butin the developing brain, CMV can cause debilitating neurodegenerationand death; studies using the CMV promoter aid in understandingthe affinity of CMV that has been suggested for specific brainregions.

Key words: green fluorescent protein; development; cytomegalovirus; axon growth cone; cerebellum; spinal cord; olfaction; hypothalamus

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

In lower animals with simpler nervous systems, single types of cells can be recognized and studied in living and fixed neurons,particularly during development. The elegant studies on axonalgrowth and neuronal development in grasshopper (Goodman and Spitzer,1979; Keshishian and Bentley, 1983) and other species with simplesystems, including Drosophila and nematodes, have benefited significantlyfrom being able to identify repeatedly selected cells and theiraxons in related experiments. To allow some of the same advantagesin the mammalian brain, we generated transgenic mice that havestrong expression of a marker gene, green fluorescent protein(GFP), that is expressed throughout the processes in restrictedsubpopulations of neurons in the brain and spinalcord.

Viral vectors that express GFP have been used to label neurons, but some viruses have the problem of being potentially toxic,and virally induced GFP is generally transient (Moriyoshi et al.,1996). Biolistics works nicely to shoot GFP gene-coated particlesinto brain slices, but which cell expresses the gene is partiallyrandom, and biolistics does not work well with cultured cells(Lo et al., 1994).

In some previous experiments, the intensity of GFP expression has not been particularly strong. This is a problem for experimentsin which one needs to study axonal growth over an extended timeperiod and needs to strongly label the neuritic arbor. Neuronsthat were genetically engineered to express the GFP gene continuously,both in vivo and in vitro, would be an asset in studies of neuronalgrowth and response to injury. We have generated such a system,as describedbelow.

Transgenic mice expressing a histochemical label have provided an important tool for the identification of neurons in theCNS. The lac Z gene coding for bacterial $beta$ -galactosidase has beenused with a number of promoters and works well to identify positivecells but requires histochemical reaction generally on dead cells(Forss-Petter et al., 1990; Jankovski and Sotelo, 1996; Paradieset al., 1996; Sekerkova et al., 1997). Furthermore, in most cases,the reaction product is restricted to the region of the cell body,making it of limited use for studies of axonal projections anddendritic architecture. An interesting alternate approach to studylive cells has been to generate transgenic mice that express anenzyme, such as alkaline phosphatase, on the outer surface oflive cells (Gustincich et al., 1997), but this still requireshistochemical reaction to identify positivecells.

We have generated transgenic mice that express an enhanced form of the jellyfish GFP protein that has been codon-corrected(from jellyfish to human) and red-shifted (Phe64 to Leu and Ser65to Thr) under control of part of the human cytomegalovirus majorimmediate early promoter (here referred to as CMV promoter). Previousreports have used other reporter genes to study viral promotersto determine the relevance of the promoter to selective patternsof viral infection in the brain (Kothary et al., 1991; Koedoodet al., 1995; Fritschy et al., 1996). Our transgenic mice showa strong expression of GFP in a limited subset of neurons, andthe same cell types express GFP from one generation to the next.The axons of these cells are strongly labeled to their terminals.A benefit of expression limited to a small number of neurons isthat this allows a focus on subsets of neurons that may behavesimilarly, whereas other neurons in the same region of the brainor spinal cord are rendered invisible. GFP can be detected inthe living cell bodies and throughout the entire extent of theliving or fixedaxons.

The significant advantage of this transgenic mouse for studying neuronal development and physiology is that a small subsetof neurons can be recognized and studied by virtue of their GFPexpression in vivo and in vitro. GFP has no apparent physiologicaleffect, and GFP-expressing cells look, behave, and develop thesame as non-GFP cells. This strategy of using transgenic micewith strong GFP expression in a very restricted subset of neuronsin the developing and mature brain should be a significant aidfor addressing a number ofquestions.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Neuronal transfection with GFP cDNA. We used a GFP cDNA variant (Clontech, Palo Alto, CA) that was shifted in the red direction(longer wavelength) and corrected from jellyfish (Chalfie et al.,1994) to mammalian codon with improved fluorescence (Chalfie,1995; Heim and Tsien, 1996; Yang et al., 1996). Two amino acidmutations were used (Phe64 to Leu and Ser65 to Thr). Neurons fromnormal nontransgenic mice were transfected with a Life Technologies(Gaithersburg, MD) Cell Porator electroporator. The electroporatorwas placed on a Gyrotory Shaker rotary table to increase fluidmotion in the cuvette and was used with a 60 µF pulse at roomtemperature. Four million cells were placed in 0.4 ml of buffer,together with 10-80 µg of GFP cDNA. After electroporation, cellswere gently centrifuged to remove the DNA-containing supernatantand then plated on polylysine-coated coverslips. In other experimentsbelow, neurons from GFP transgenic mice were used, which had theGFP sequence incorporated into their genome and did not requirefurther labeling ortransfection.

Preparation of the DNA transgene. The pEGFP-C1 plasmid vector from Clontech was propagated in Escherichia coli DH5 $alpha$ in thepresence of kanamycin (30 µg/ml). pEGFP-C1, a C-terminal proteinfusion vector, contains an enhanced jellyfish GFP. The GFP isunder the control of a strong major immediate early promoter fromthe human CMV promoter. The vector DNA was isolated and bandedtwice over a CsCl-ethidium bromide gradient by equilibrium centrifugation.The purified vector DNA was digested with the restriction enzymesNsi-1 and Mlu-1, with appropriate buffers. The Nsi-1- and Mlu-1-digestedDNA was subsequently electrophoresed on a 1% agarose gel withtetraethylammonium buffer to isolate a 1.642 kb fragment containingthe CMV immediate early promoter sequence ( $-$ 583 to +7 of the CMVpromoter sequence), the enhanced GFP sequence, multiple cloningsites, and SV40 poly(A)signals.

DNA preparation for microinjection. The 1.6 kb DNA fragment containing the GFP coding sequence with the CMV promoter and SV40poly(A) signal was purified from the agarose gel by the QIAquickgel extraction kit protocol from Qiagen (Hilden, Germany). Theprecipitated DNA was pelleted, washed, air dried, and then purifiedand concentrated by passing through a Schleicher & Schuell (Keene,NH) Elutip-d column and then through three Millipore (Bedford,MA) VMWP01300 filters. After dialysis, the DNA was collected,and the concentration was determined by optical density and adjustedto 5 ng/µl with injection buffer. Before microinjection, the DNAwas filtered through a 0.45 µm Millipore SJHV004NS syringefilter.

Generation of transgenic mice. Fertilized mouse oocytes were isolated from the F2 generation of matings between female andmale (C57B1/6 XC3H/HEJ) mice. The purified DNA with a concentrationof 1-2 ng/µl was injected into the fertilized oocytes. After microinjection,the oocytes that survived were transplanted to the oviducts ofpseudopregnant B6C3 F2 strain of foster mothers. The transgenicmice expressing the GFP gene were identified by PCR from DNA isolatedfrom tail biopsies by using GFP-specific forward and reverse primers.Tail tissue was digested with 500 µg/ml proteinase K in 700 µlof buffer containing 50 mM Tris-HCl, pH 8.0, 100 mM EDTA, and0.5% SDS at 55°C overnight with agitation. The DNA was precipitatedfrom the aqueous phase by adding 0.1 vol of 3 M NaAc, pH 6.0,and 2 vol of ethanol at room temperature. After pelleting, theDNA was washed with 70% ethanol to remove traces of phenol andSDS. The concentrations of the DNA from different samples wereequalized after measurement of opticaldensity.

In our studies of 45 potential founder mice, 15 incorporated the GFP sequence in their genomes. These 15 founder mice werebred, and their offspring was tested by a combination of PCR,analysis of brain sections for GFP in a fluorescence microscope,and examination of GFP expression in cultured neurons. Of thesemouse lines, we focus on one that showed strong GFP expressionand to a lesser extent on a second line. GFP expression is foundin the same regions of the brain and spinal cord in five generationsof thesemice.

PCR detection of transgenic mice expressing GFP. Two synthetic oligomers, one forward primer 5'-TAA ACG GCC ACA AGT TCA GC-3'and one reverse primer 5'-TGT TCT GCT GGT AGT GGT CG-3' were madefrom GFP coding sequences and used for PCR amplification of transgenicmouse DNA templates. The PCR reactions were performed in 50 µlwith 50 ng of transgenic DNA, each with 10 mM Tris, pH 8.3, 50mM KCl, 1.5 mM MgCl₂, 200 µl each of dATP, dGTP, dCTP, and TTP,50 ng each of forward primer and reverse primer, and 1 U of AmpliTaqDNA polymerase. The PCR reactions were done as follows: denaturationat 94°C for 5 min, 94°C for 1 min, 55°C for 1 min, and 72°C for2 min for 40 cycles. For a positive control, PCR was also performedon the GFP DNA fragment (Nsi-1 plus Mlu-1 fragment), which wasoriginally introduced into the oocytes to generate transgenicmice. A negative control without DNA was performed also. The PCRreactions were analyzed on a 1% agarose gel to look for positivetransgenic mice. An expected DNA band migrating at 472 bp positionwas observed in the positive control and in lanes containing GFP-positivetransgenic mouse DNA but not in the negative controllanes.

mRNA analysis of different tissues obtained from transgenic mice expressing GFP. A number of different tissues from two transgenicmice were harvested, and total RNA was extracted with TRIZOL (LifeTechnologies). Different tissues included several different brainregions and non-neuronal tissue. Approximately 10 µg of totalRNA was loaded from each sample for Northern blots. A GFP DNAfragment was used as a probe for Northern blots. A cyclophilinprobe was used as a control for relative loading of each lane.After detection of GFP RNA, the Northern blot was stripped andprobed again for cyclophilin (van den Pol et al., 1994).

GFP detection. The use of PCR to detect the GFP transgene was sensitive in this regard but did not establish that the proteinwas actually expressed. To determine which mice showed GFP expressionduring development of this transgenic line, we used unfixed freshtissue sections of GFP transgenic mice. Sections were cut on avibratome. Fresh sections worked well, except that cells thatwere cut open tended to leak GFP, which raised the backgroundfluorescence; for this reason, we observed some fresh sectionswhile perfusing with a HEPES buffer to wash out leaky GFP. Insome cases, before death, we viewed deeply anesthetized mice underthe fluorescent microscope or took whole pieces or parts of thebrain or spinal cord for viewing. In addition, we also used tissueculture of brain cells from postnatal day 1 mice to determinewhich founder lines expressed the transgene. Four mice per litterwere pooled, and neurons were plated on glass coverslips. If GFP-positivecells were detected in the next 3 d, then the founder mouse ofthat line was used for subsequent breeding. If the cells werenegative, the founder mouse was not usedfurther.

Because GFP tended to leak out of unfixed cells that were cut during histological processing, particularly obvious in thinnersections, some mice were aldehyde-fixed. Under deep sodium pentobarbitalanesthesia, mice (n = 12) were perfused with 4% paraformaldehyde,and the brains were removed and cut on a vibratome or freezingmicrotome into 30-40 µm sections. GFP was still visible afterfixation without immunostaining, although the relative intensityof fluorescence was decreased by the aldehyde. To overcome thealdehyde-mediated reduction in GFP fluorescence, a GFP antiserum(Clontech) was used with peroxidase immunocytochemistry to stainsome sections. The primary rabbit antiserum was used at a 1:2500dilution and was visualized with goat anti-rabbit IgG-biotin andthen by avidin-biotin-peroxidase immunostaining using reagentsfrom Vector Laboratories (Burlingame, CA), followed by treatmentwith diaminobenzidine and hydrogen peroxide, as described elsewhere(van den Pol, 1985). Only transgenic mice showed brown peroxidaselabeling, and it was found in the same brain regions in whichGFP fluorescence was found. Staining with immunoperoxidase allowedthe long-term storage and analysis of sections from GFP transgenicbrains and the potential for later use for electronmicroscopy.

GFP expression was detected and photographed with Olympus Optical (Tokyo, Japan) and Zeiss (Oberkochen, Germany) fluorescentmicroscopes. An inverted Olympus IX70 with a 150 W mercury arclamp with a fluorescein filter set gave the best GFP signal. ABio-Rad (Hercules, CA) 500 confocal scanning laser microscopewith an argon laser was also used to examine thick tissue sections.Some of the photomicrographs presented here are digital imagesfrom photographic negatives scanned on an Eastman Kodak (Rochester,NY) slide scanner and printed on an Eastman Kodak 7700 or 8650dye sublimationprinter.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Neuronal transfection

Before generating transgenic mice, we examined intensity and distribution of fluorescence with GFP-coding DNA from differentplasmids after transfection of primary neurons with electroporationin >500 cultures. Previous studies with cotransfection experimentshave shown that GFP can be used as a reporter for neuronal genestransfected into non-neuronal cells in vitro (Marshall et al.,1995). We compared actin, immediate early CMV, and mouse prionpromoters. GFP-coding DNA from several different plasmids werecompared with lac Z-coding plasmids using the same promoters.Transfection with lac Z yielded nicely labeled neuron cell bodiesbut poorly labeled axons and distal dendrites. In contrast, transfectionwith plasmids containing the enhanced GFP gave the strongest signal,and GFP fluorescence was found throughout the cytoplasm, includingin axons and dendrites (Fig. 1A). Neurons from all areas used,including mouse, rat, and human neurons from olfactory bulb, hypothalamus,hippocampus, cortex, and spinal cord, showed strong labeling.Glial cells were also labeled in transfection experiments (Fig.1B); because the glial cells divided in culture, the GFP labelwas diminished in daughter cells. We also used recombinant DNAfrom plasmids made in which GFP was tethered to the axonal proteintau, with the cDNA coding for tau inserted at the C-terminal endof GFP. Neurons transfected with the tau-GFP construct showedgreen label in some of their processes, but the intensity of labelingwas less, and the distribution was restricted. Within single neurons,both long-branching axons and dendrites were less strongly labeledwith tau-GFP compared with neurons transfected with GFP alone.Although the efficiency of any particular promoter for expressionin transfected neurons may not parallel its efficiency in thebrains of transgenic animals, based on the strong levels of expressionand the widespread intracellular distribution of GFP with theCMV-GFP construct, we selected this construct to generate transgenicmice. Because the CMV itself appears to preferentially infectsubsets of neurons in the brain (Ho, 1991), we reasoned that itspromoter might behave similarly in transgenic animals and generatehigh levels of GFP expression in subsets of neurons.

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Figure 1. GFP transfected neurons. A, Two neurons with their neurites expressing GFP 2 d after transfection by electroporation. Scale bar, 12 µm. B, A cell with the appearance of a glial cell is seen after GFP transfection. Scale bar, 10 µm.

Transgenic mice with GFP expression in restricted populations of neurons

Examination of the brains and spinal cords of transgenic mice revealed expression of GFP in restricted types of neurons fromthe olfactory bulb to the sacral spinal cord. GFP appeared tobe expressed by similar types of neurons within any single regionand appeared to be constant from one generation of mice to thenext. We estimate that the number of types of neuron that expresseddetectable GFP was <3%. GFP could be detected in freshly cut sectionsviewed in a fluorescent microscope or laser confocal microscope,or after fixation and immunoperoxidase staining. Immunoperoxidaserevealed cells and processes in the same regions as seen withfluorescent microscopy and allowed the use of differential interferencecontrast (DIC) microscopy, which facilitated detection of unlabeledcells in the background. Some types of neurons showed very strongexpression that revealed the entire neurons, including the cellbody (Fig. 2A,C-E), dendrites and their filopodia (Fig. 2B), andaxons and their terminal boutons (Figs. 3A-G, 4, 5A-C). GFP-positivecells were found in the hypothalamic suprachiasmatic nuclei (datanot shown); little labeling was found in the lateral hypothalamus.The large cells of reticular gigantocellularis showed GFP. Inother regions of the brain, neurons were found with less robustGFP expression, such as in the CA3 region of the hippocampus,in a subpopulation of striatal neurons, and in the medial nucleusof the trapezoid body. Cells with the appearance of glial cellsshowed little GFP. In contrast, GFP expression via adenovirusintroduction of the GFP gene into the CNS appeared to be foundprimarily in glial cells, although neuronal labeling was alsonoted (Moriyoshi et al., 1996). An asset of the approach we usedis that GFP label is found not only in the cell bodies of livingand fixed tissue, but it also can label distal axonal and dendriticprocesses. In previous studies of other transgenic mice whichused different regions of the CMV promoter sequence, there waslittle or no detectable reporter gene in neuronal processes. Thiswas attributable to the use of nuclear localization signals (Koedoodet al., 1995; Fritschy et al., 1996), the use of lac Z ratherthan GFP (Baskar et al., 1996), and potentially to differencesin the promoter sequence used in each study.

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Figure 2. GFP in cell bodies and dendrites. A, Cells labeled with GFP immunoperoxidase in medulla. Scale bar, 20 µm. B, Long spine-like processes show GFP fluorescence, as shown in this example from the granule cell region of the olfactory bulb. Scale bar, 4 µm. C, Under the cerebellum (crb), neurons in the vestibular complex show GFP expression in cell bodies and dendrites. D, Higher magnification of C. Scale bar, 25 µm. E, In the spinal cord, motoneurons in the ventral horn of this sagittal section express GFP. Scale bar, 35 µm.

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Figure 3. GFP in axons and their terminals. A, In the cochlear nuclei, some axons show strong GFP fluorescence and have terminal boutons. Scale bar, 2 µm. B, In the cerebellar cortex, GFP-expressing mossy fibers in the white matter enter the cerebellar cortex before spreading out to innervate the granule cell region. Scale bar, 10 µm. C-E, Mossy fiber terminals in the granule cell layer after GFP immunoperoxidase staining. Background visualization of granule cells is aided by DIC microscopy. C, Arrows show moss-like shape typical of these fibers. D, A later generation of transgenic mice shows a similar expression of GFP in the mossy fiber. E, A different line of transgenic mice with the same CMV promoter sequence as in C and D shows the same patterns of labeling, as shown here by the labeled mossy fiber. Scale bar (in C): C-E, 5 µm. F, In spinal cord, fibers make terminal boutons (arrows) in the gray matter (GM) after leaving the white matter (WM). Scale bar, 9 µm. G, In dorsolateral cervical spinal cord white matter, long axons can be followed for many millimeters. Scale bar, 5 µm.

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Figure 4. Parasagittal bands of GFP in cerebellar mossy fibers. In this low-magnification micrograph, GFP-expressing mossy fibers are found in parasagittal bands (arrows) in this coronal section of the cerebellum. Only mossy fibers are labeled here. Scale bar, 35 µm.

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Figure 5. GFP in axons. A, In a sagittal section of the midbrain, GFP-containing axons detected with immunoperoxidase have many labeled terminal boutons. No cell body labeling is seen in this area. B, In the living dorsal root, GFP fluorescent axons emerging from the DRG (right) are found (arrows). Scale bar, 4 µm. C, Five days after spinal cord dorsal column damage in the transgenic mouse, ascending GFP axons in the dorsal column begin to show small filopodia. GFP axon is immunostained with peroxidase in this horizontal section of midthoracic spinal cord. Scale bar, 4 µm.

GFP was expressed in a group of ~5-15% of the neurons in the dorsal root ganglia and in the axons from the DRG (Fig. 5B) thatrun rostrally up the dorsal columns of the cord (Fig. 5C). Alldorsal root ganglia studied appear to have GFP-expressing neurons.Some large, strongly fluorescent neurons were found in the ventralhorn in motoneurons (Fig. 2E). GFP was detected in the dorsalcolumns of the intact in situ spinal cord and in the associateddorsal root ganglia and dorsal root (Fig. 5B) when deeply anesthetizedmice were placed on a microscope before fixation perfusion. Axonswere found in the white (Fig. 3G) and gray (Fig. 3F) matter. Todemonstrate that GFP was expressed in experimental damaged spinalcord axons, we cut the right side of the dorsal columns of 8-week-oldtransgenic mice with a shallow penetration of a number 11 scalpelblade into the thoracic spinal cord. Five days after sectioning,the ascending part of GFP-expressing DRG axons in the dorsal columnshowed small lateral GFP fluorescent filopodia, suggestive ofgrowth (Fig. 5C) not commonly seen in control cord. This indicatesthat GFP expression in the axons of the spinal cord of the transgenicmice may be useful for studying axonal responses toinjury.

The olfactory bulb showed the highest level of GFP expression within the brain. In Northern blots examining GFP mRNA expression,the olfactory bulb showed a higher level of GFP expression thanany other brain or nonbrain tissue (Fig. 6). The expression wasrestricted primarily to the small inhibitory cells of the bulbthat are immunoreactive for the transmitter GABA. Most granulecells showed GFP expression. In addition, juxtaglomerular cellsshowed GFP expression. Other cells of the bulb, particularly theexcitatory mitral or tufted cells, showed no GFP. Some of theolfactory glomeruli showed strong expression (Fig. 7B), and othersshowed weak expression (Fig. 7B). This suggested that subpopulationsof olfactory receptor cells that terminate in the glomeruli expressedGFP. This was consistent with patches of olfactory axons showingGFP and olfactory receptor cells in the olfactory mucosa expressingGFP (Fig. 7C).

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Figure 6. Northern blot of GFP expression. RNA was extracted from various tissues of transgenic mice and probed on a Northern blot for GFP. The highest level of expression was in the olfactory bulb. Other brain regions showed lower levels of expression. Brain refers to the remaining brain after the other regions in the blot were removed. After stripping, as a control, the blot was probed with cyclophilin to demonstrate the general level of RNA loading in each lane.

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Figure 7. Olfactory bulb GFP. A, In the olfactory bulb, two unusual neurons (large arrows) showing strong GFP expression were immunostained with GFP immunoperoxidase. Axons (small arrow) can sometimes be followed from the cell body down into the granule cell layer. GL, Glomerular layer; EPL, external plexiform layer; GCL, granule cell layer. Scale bar, 35 µm. B, In olfactory bulb, some glomeruli (long arrows) show strong GFP immunoperoxidase. Other glomeruli (short arrows) show little staining. Scale bar, 70 µm. C, In the olfactory mucosa of a developing mouse on the day of birth, some olfactory receptor cells, together with their sensory dendrite and efferent axons (small arrows), show GFP expression, consistent with the labeling of some glomeruli shown in B. Unlabeled background cells are seen with DIC microscopy. Scale bar, 15 µm.

The strongest expression of GFP in the bulb was found in an unusual type of cell in the external plexiform layer (EPL); cellbodies were found from the most external part of the granule celllayer through the EPL (Fig. 7A). These cells had dendritic arborswith one to four primary dendrites, which divided two or threetimes and remained in the EPL or near the external zone of theEPL. Many long spine-like appendages arose from the dendritesand ended in small swellings. The cell body of these cells waslarger than that of typical granule cells and had an axon arisingfrom the cell body and going in a direction toward the granulecell layer, suggesting these were not displaced granule cellsthat have no axon. A common cell of the EPL is the tufted cell,but that cell does not have dendritic spines, and the tufted celldendrites enter the glomerular layer and form a distinctive tuft(Mori, 1987; Shepherd and Greer, 1990) not seen in the GFP-labeledcells. Another type of cell in the EPL is the van Gehuchten cell(Shipley et al., 1995). These cells contain vasoactive intestinalpolypeptide, peptide histidine isoleucine, and other antigens(Sanides-Kohlrausch and Wahle, 1990; Alonso et al., 1993). However,descriptions of these van Gehuchten cells suggest they have localaxon collaterals in the EPL and do not appear to have extensivedendritic spines, unlike the cells described here. Thus, the stronglyGFP-positive cells in the EPL do not fit into any clear descriptionof previously characterized neuronshere.

Little GFP was found in the cell bodies of the cerebellar cortex. However, GFP was found in a subset of mossy fibers (Fig.3B) and their terminals (Fig. 3C-E), originating outside the cerebellum,that provide excitatory innervation to the granule cells. Notall mossy fibers were GFP-positive, indicating that only a subsetof the neurons that send mossy fiber projections to the granulecells expressed GFP. In coronal sections, GFP-expressing mossyfibers were found in parasagittal bands (Fig. 4), particularlyobvious in the vermis. Mossy fibers are unique axons that makelarge terminal endings covered with small moss-like short appendages,and these showed robust GFP expression (Fig. 3C-E). Climbing fibers,the other primary excitatory afferent input to the cerebellarcortex, did not express GFP. The description here is not an exhaustivesurvey of all neurons that express GFP in these transgenic micebut instead delineates some of the major groups and serves asanoverview.

In a second transgenic line made with the same CMV-GFP construct, the distribution of GFP-expressing neurons was similar tothat described above, and the relative intensity of GFP expressionin positive neurons was also parallel. An example of this stainingin the second transgenic line is the absence of positive GFP cellbodies in the cerebellar cortex but the expression of GFP in cerebellarmossy fibers (Fig. 3E). Each line showed some variability betweenanimals in levels ofexpression.

Developing brain

The level of GFP expression was stronger in developing brains that in adults. GFP expression was well developed in embryonicbrains (data not shown). This is parallel to the high infectionrates of the virus in the developing brain compared with the adultand supports the idea that the CMV (immediate early) promotermay be maximally activated in developing neurons. Embryonic day18 and postnatal day 1 brains still in the head were sectionedand examined with or without immunostaining with GFP antisera.The strongest expression in these animals, as in adults, was foundin the olfactory system in which early granule cells and juxtaglomerularcells expressed GFP, and olfactory receptor cells in the mucosa,together with their axons projecting into the bulb, were alsolabeled (Fig. 7C). In other regions of the brain in which positiveneurons were found, the level of expression appeared higher atearlier stages ofdevelopment.

Tissue culture of neurons from GFP transgenic mice

Different regions of brains or spinal cords from GFP transgenic mice were cultured. In strongly expressing transgenic cellsin vitro, the GFP fluorescence was very bright and could be seeneasily by eye, even with a 10× microscope objective. Because GFPdoes not easily fade and is remarkably stable, even during photoactivation,labeled living cells could be drawn with a camera lucida, photographed(Fig. 8), and then returned to the incubator. The entire axonaland dendritic arbor of single neurons could be clearly visualized.This was verified by examining single neurons growing on a glasssubstrate and by comparing the GFP fluorescent image with video-enhancedDIC microscopy. Every part of the neuritic tree that could beseen with the DIC image was also fluorescently labeled. Furthermore,there was no decrease in the intensity of fluorescence from proximalto distal, demonstrating that the entire neuritic tree was labeledwith GFP. Both dendritic and axonal processes were well labeled,including their filopodia, lamelipodia, and terminal boutons.In developing neurons, both dendritic and axonal growth coneswere clearly labeled. GFP expression was detected in positivecells as soon as they were plated. Regions of the brain, suchas the olfactory bulb, with high number of positive cells alsoshowed large numbers of positive cells in culture, whereas negativebrain regions, such as the cerebellar cortex, did not. Immunostainingwith Alexa 546 [a red fluorescent immunolabel from Molecular Probes(Eugene, OR)] showed glutamate decarboxylase immunoreactivity(antisera from Dr. W. Oertel) (van den Pol, 1985) in the GFP-expressingcells of cultured olfactory bulb neurons, consistent with theGABAergic identity of the transmitter of granule cells and thelocation of GFP-expressing cells in tissue sections of the olfactorybulb.

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Figure 8. GFP in cultured spinal cord neurons. After 4 d in vitro, a few neurons show strong GFP expression, even at their smallest filopodia. Inset, Arrow shows same small growth process. GFP fluorescence is found in cell bodies and all processes. Other cells in the same field show little fluorescence. Scale bar, 6 µm.

  DISCUSSION

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Potential use of transgenic mice with selective GFP expression

We demonstrate here that GFP is expressed selectively by subsets of neurons in the brain and spinal cord in adult and developingbrain. In cells that strongly express GFP, their entire dendriticand axonal arbor is labeled. The potential advantage of this approachto labeling neurons is that in each generation the same neuronsand their processes are labeled, allowing ongoing physiologicaland structural studies. Developing mice expressing GFP selectivelyin subpopulations of neurons may also be helpful for determinationof cell lineage and fate maps of dividing cells during development.In parallel, the development of growing axons can be studied duringdevelopment and after injury, in both fixed and living tissue.Cells that express GFP in situ also express GFP in vitro, allowingrecognition of specific subsets of green cells in culture, ofpotential importance for characterization of the electrophysiologyor single cell molecular biology of identified cells. Neuronsexpressing GFP are also ideal for transplantation studies in whichboth the cells and their processes could be followed in the non-GFPhost brain. Finally, as described below, slight changes in theCMV (immediate early) promoter sequence may allow other populationsof neurons that do not express GFP in the present study to generatehigh levels of GFP in other transgenicmice.

To study axons, their growth, and response to injury, the axon must be visualized. This can be achieved by applying a dye,such as DiI, to the outside of the cell, and this works well insome experiments; however, these dyes are often not strong enoughto label thin distant axon terminals for extended periods (Liljelundet al., 1994). Alternately, labels such as neurobiotin or biocytin(Horikawa and Armstrong, 1988), or fluorescent molecules, suchas fluorescent dextran, can be injected by a micropipette directlyinto a cell, labeling the entire dendritic arbor and axon trajectory.Although biocytin works well to label the entire cell, the processis labor-intensive, because the cell must be injected, fixed,and the stained, and labeled processes cannot be visualized whilealive. Injection of fluorescent molecules works well for shorttime intervals, but the dye is usually degraded after a few daysor sequestered in lysosomes and no longer labels the entire neuritictree. Some dyes, such as Lucifer yellow, may even be toxic tothe cell when viewed under fluorescent light. In contrast, intransgenic mice with strong GFP expression, axons are well labeledover long periods of time, and even filopodia on growing axonsand terminal boutons on mature axons are strongly labeled, attributable,in part, to the ongoing synthesis of the GFP molecule. Furthermore,because only small subsets of neurons are labeled, individuallive or fixed axons and dendrites can be followed in their entiretybecause of the transparency of cells that do not express GFP,which constitute the greatmajority.

The GFP transgenic mice described here can be crossbred with one of the many interesting mutant mice that have been used previouslyfor studying development, particularly in the cerebellum (Rakic,1979). Because our transgenic mice have strong GFP expressionin subsets of mossy fibers that innervate select parasagittalregions of the cerebellum, crossing these with mutants that haveintrinsic defects in cerebellar development may prove a usefulmodel for studying specificity of axonal target recognition. Inparallel, crossing our mice with knock-out or overexpressing transgenicmice may provide a window for studying the contribution of specificgenes involved in axonal growth of specific circuits that expresstheir own label in living and fixedtissue.

When a label is introduced into the brain, either via direct injection, chemical manipulation, or viral mediation, the cellslabeled may vary from experiment to experiment. In contrast, inthe transgenic mice, the same populations of cells are labeledfrom generation to generation. Importantly, the CMV promoter isexpressed at very early stages of brain development (Kothary etal., 1991; Koedood et al., 1995), allowing studies of cell division,migration, and process outgrowth in identified cells in the mammalianbrain.

CMV immediate early promoter

CMV is a virus that probably infects the majority of adult humans (Ho, 1991). In most cases, it remains latent and accountsfor little debilitation. In striking contrast, in the developinghuman brain, CMV infection can be disastrous. Early human braininfection with CMV, found in several thousand infants born eachyear, can lead to microencephaly, deafness, retardation, and seizures(Saigal et al., 1982; Ho, 1991; Perlman and Argyle, 1992). Similarproblems in infected adults are not found unless the immune systemis compromised, as with HIV infection (Nelson et al., 1988; Wileyand Nelson, 1988), and then CMV has been considered to be a significantthreat. One factor that leads to the greater CMV problem in developingbrains has been attributed to the fact that the immune systemis not sufficiently developed to counteract CMV spread. Anotherfactor is that developing neurons may allow higher levels of expressionof the CMV promoter. The major immediate early CMV promoter drivesthe expression of two early CMV genes that set the stage for viralreplication; enhanced expression of the promoter in developingneurons may constitute an additional mechanism for the greaterdebilitation found in developing humans. This concept is supportedby the results from both the present paper and other works (Kotharyet al., 1991; Koedood et al., 1995), showing that the CMV promoteris most active in early development, the same period when thevirus is most active in thebrain.

As we described in Results, the CMV promoter (Boshart et al., 1985) works well to drive GFP expression in all neurons transfectedin vitro with a GFP-containing plasmid DNA and generates brightlylabeled cells. In contrast, in the transgenic mice with the sameCMV promoter sequence, GFP expression was highly localized tospecific neuronal groups, indicating the same CMV promoter sequenceacted differently in transgenic and transfectedneurons.

Different sequences of the CMV promoter have been used previously with a lac Z reporter with a nuclear localization site (Koedoodet al., 1995; Fritschy et al., 1996). Because of the nuclear localizationand necessity of staining with a suitable colorant such as X-gal,those mice were less suitable for studies of living neurons thanthe GFP mice we describe here. What is of potential significantinterest is that with slight changes in the CMV promoter sequence,many of the cells that express the reporter gene are quite different.For instance, previously with a $-$ 524 to +13 human CMV promoter,expression was found in the mitral cells of the olfactory bulb,retina, CA1 region of the hippocampus, and the granule cells ofthe cerebellum (Fritschy et al., 1996). In contrast, in the transgenicmice described here with a $-$ 583 to +7 CMV promoter sequence, wefound no expression in any of these cells but did find expressionin other cells in the same areas. We found little retinal expression.In the olfactory bulb, we found no labeled excitatory mitral cellsbut did find many labeled inhibitory granule and juxtaglomerularcells. In the hippocampus, we found no labeled CA1 cells but didfind some CA3 labeling. In the cerebellar cortex, we found nolabeled cells at all but found striking expression in a subpopulationof mossy fibers that originate outside the cerebellar cortex andterminate in the granule cell region. We also found weak expressionin the striatum in which no expression was found with the $-$ 524to +13 CMV promoter sequence used by Fritschy et al. (1996).

It might be argued that the difference between the studies is simply because of the random site of integration into chromosomes.This, however, seems less likely, because in our study we generatedtwo independent transgenic lines, made with the same CMV promotersequence, that showed almost identical sites of expression inthe CNS. Similarly, in a previous study with the CMV promoter(Kothary et al., 1991), two different transgenic lines expresseda reporter gene in the same regions of the mice in that studybut different from the loci expressing in our mice. Koedood etal. (1995) also reported that transgenic mice with $-$ 524 to +13of the CMV promoter showed patterns of expression that were similarin all three lines studied; similar to other investigators, theyfound the total levels of expression varied between lines, possiblyrelated to different sites of integration. The difference in lociof expression could also be attributable to differences in themouse strains used; however, we started out with a cross betweentwo pigmented strains to generate the founder transgenic mice,and when we outcrossed these to albino mice, the loci of expressionremained the same, suggesting that strain differences do not easilyaccount for substantial differences. Furthermore, we used C57Bmice as part of our initial strain, similar to Kothary et al.(1991). Kothary found expression in muscles and retina and littlein brain, whereas we found strong expression in some brain regionsand little in retina ormuscle.

In three transgenic mouse lines with lac Z expression, under control of $-$ 670 to +54 human CMV promoter, tissue distributionwas similar between the three lines (Baskar et al., 1996). Tissueexpression of lac Z, not limited to the brain, was also foundto be similar to each other in two transgenic mice with a $-$ 302to +72 CMV promoter (Kothary et al., 1991). That different regionsof the CMV promoter would generate different patterns of expressionin CNS neurons is consistent with the complexity of the CMV promoterthat contains binding sites for cAMP, CREB/ATF, NF-KB, SP1, YY1,retinoic acid, AP-1, NF1, methylation, and its own immediate earlyprotein product (Ghazal et al., 1988, 1992; Hunninghake et al.,1989; Meier and Stinski, 1996, 1997; Mocarski et al., 1996; Proschet al., 1996).

Another approach to generating transgenic mice in subpopulations of neurons is to use promoters that are specific for substancesexpressed in subtypes of neurons, such as a neurotransmitter orits synthetic enzymes (Liu et al., 1997). This approach has beenused and should also prove useful. However, the level of expressionin positive cells may not be as high as with the CMV promoter,and transmitter promoters may be expressed by cells normally notusing a particular transmitter, as described for lac Z expressionunder control of the 5' regulatory region of the glutamate decarboxylase-67promoter in non-GABAergic excitatory neurons (Sekerkova et al.,1997).

  FOOTNOTES

Received July 14, 1998; revised Sept. 9, 1998; accepted Sept. 28, 1998.

This work was supported by the National Science Foundation and National Institutes of Health Grants NS34887 and NS31573. Wethank Y. Yang for excellent expert help with these experiments,and Drs. E. Mocarski and R. Flavell for helpful suggestions relatingto CMV and transgenicmice.
Correspondence should be addressed to Anthony N. van den Pol, Department of Neurosurgery, Yale University School of Medicine,333 Cedar Street, New Haven, CT06520.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Alonso JR, Arevalo R, Porteros A, Binon JG, Lara J, Aijon J (1993) Calbindin D-28K and NADPH-diaphorase activity are localized in different populations of periglomerular cells in the rat olfactory bulb. J Chem Neuroanat 6:1-6[ISI][Medline].
Baskar JF, Smith PP, Nilvar G, Jupp RA, Hoffmann S, Peffer NJ, Tenney DJ, Colberg-Poley AM, Ghazal P, Nelson JA (1996) The enhancer domain of the human cytomegalovirus major immediate-early promoter determines cell type-specific expression in transgenic mice. J Virol 70:3207-3214[Abstract].
Boshart M, Weber F, Jahn G, Dorsch-Hasler K, Fleckenstein B, Schaffner W (1985) A very strong enhancer is located upstream of an immediate early gene of human cytomegalovirus. Cell 41:521-530[ISI][Medline].
Chalfie M (1995) Green fluorescent protein. Photochem Photobiol 62:651-656[ISI][Medline].
Chalfie M, Tu Y, Euskirchen G, Ward WW, Prasher DC (1994) Green fluorescent protein as a marker for gene expression. Science 263:802-805[Abstract/Free Full Text].
Forss-Petter S, Danielson PE, Catsicas S, Battenberg E, Price J, Nerenberg M, Sutcliffe JG (1990) Transgenic mice expressing beta-galactosidase in mature neurons under neuron-specific enolase promoter control. Neuron 5:187-197[ISI][Medline].
Fritschy JM, Brandner S, Aguzzi A, Koedood M, Luscher B, Mitchell PJ (1996) Brain cell type specificity and gliosis-induced activation of the human cytomegalovirus immediate-early promoter in transgenic mice. J Neurosci 16:2275-2282[Abstract/Free Full Text].
Ghazal P, Lubon H, Heninghausen L (1988) Specific interactions between transcription factors and the promoter-regulatory region of the human cytomegalovirus major immediate-early gene. J Virol 62:1076-1079[Abstract/Free Full Text].
Ghazal P, DeMattei C, Giulietti E, Kliewer SA, Umesono K, Evans RM (1992) Retinoic acid receptors initiate induction of the cytomegalovirus enhancer in embryonal cells. Proc Natl Acad Sci USA 89:7630-7634[Abstract/Free Full Text].
Goodman CS, Spitzer NC (1979) Embryonic development of identified neurons: differentiation from neuroblast to neurone. Nature 280:208-214[Medline].
Gustincich S, Feigenspan A, Wu DK, Koopman LJ, Ravioli E (1997) Control of dopamine release in the retina: a transgenic approach to neural networks. Neuron 18:723-736[ISI][Medline].
Heim R, Tsien RY (1996) Engineering green fluorescent protein for improved brightness, long wavelength, and fluorescent resonance energy transfer. Curr Biol 6:178-182[ISI][Medline].
Ho M (1991) In: Cytomegalovirus biology and infection, pp 1-440. New York: Plenum.
Horikawa K, Armstrong WE (1988) A versatile means of intracellular labeling: injection of biocytin and its detection with avidin conjugates. J Neurosci Methods 25:1-11[ISI][Medline].
Hunninghake GW, Monick MM, Liu B, Stinski MF (1989) The promoter-regulatory region of the major immediate-early gene of human cytomegalovirus responds to T-lymphocyte stimulation and contains functional cyclic AMP-response elements. J Virol 63:3026-3033[Abstract/Free Full Text].
Jankovski A, Sotelo C (1996) Subventricular zone-olfactory bulb migratory pathway in the adult mouse: cellular composition and specificity as determined by heterochronic and heterotopic transplantation. J Comp Neurol 371:376-396[ISI][Medline].
Keshishian H, Bentley D (1983) Embryogenesis of peripheral nerve pathways in grasshopper legs. I. The initial nerve pathway to the CNS. Dev Biol 96:89-102[ISI][Medline].
Koedood M, Fichtel A, Meier P, Mitchell PJ (1995) Human cytomegalovirus (CMV) immediate-early enhancer/promoter specificity during embryogenesis defines target tissue of congenital HCMV infection. J Virol 69:2194-2207[Abstract].
Kothary R, Barton SC, Franz T, Norris ML, Hettle S, Surani MA (1991) Unusual cell specific expression of a major human cytomegalovirus immediate early gene promoter-lac Z hybrid gene in transgenic mouse embryos. Mech Dev 35:25-31[ISI][Medline].
Liljelund P, Ghosh P, van den Pol AN (1994) Expression of the neural axon adhesion molecule L1 in the developing and adult rat brain. J Biol Chem 269:32886-32895[Abstract/Free Full Text].
Liu J, Merlie JP, Todd RD, O'Malley KL (1997) Identification of cell type-specific promoter elements associated with the rat tyrosine hydroxylase gene using transgenic founder analysis. Mol Brain Res 50:33-42[Medline].
Lo DC, McAllister AK, Katz LC (1994) Neuronal transfection in brain slices using particle-mediated gene transfer. Neuron 13:1263-1268[ISI][Medline].
Marshall J, Molloy R, Moss GWJ, Howe JR, Hughes TE (1995) The jellyfish green fluorescent protein: a new tool for studying ion channel expression and function. Neuron 14:211-215[ISI][Medline].
Meier JL, Stinski MF (1996) Regulation of human cytomegalovirus immediate-early gene expression. Intervirology 39:331-342[ISI][Medline].
Meier JL, Stinski MF (1997) Effect of a modulator deletion on transcription of the human cytomegalovirus major immediate-early genes in infected undifferentiated and differentiated cells. J Virol 71:1246-1255[Abstract].
Mocarski ES, Kemble GW, Lyle JM, Greaves RF (1996) A deletion mutant in the human cytomegalovirus gene encoding IE1_491aa is replication defective due to a failure in autoregulation. Proc Natl Acad Sci USA 93:11321-11326[Abstract/Free Full Text].
Mori K (1987) Membrane and synaptic properties of identified neurons in the olfactory bulb. Prog Neurobiol 29:275-320[ISI][Medline].
Moriyoshi K, Richards LJ, Akazawa C, O'Leary DDM, Nakanishi S (1996) Labeling neural cells using adenoviral gene transfer of membrane target GFP. Neuron 16:255-260[ISI][Medline].
Nelson JA, Reynolds-Kohler C, Oldstone MBA, Wiley CA (1988) HIV and HCMV coinfect brain cells in patients with AIDS. Virology 165:286-290[ISI][Medline].
Paradies MA, Grishkat H, Smeyne RJ, Oberdick J, Morgan JI, Eisenman LM (1996) Correspondence between L7-lacZ-expressing Purkinje cells and labeled olivocerebellar fibers during late embryogenesis in the mouse. J Comp Neurol 374:451-466[ISI][Medline].
Perlman JA, Argyle C (1992) Lethal cytomegalovirus infection in preterm infants: clinical, radiological, neurological findings. Ann Neurol 31:64-68[ISI][Medline].
Prosch S, Stein J, Staak K, Liebenthal C, Volk HD, Kruger DH (1996) Inactivation of the very strong HCMV immediate early promoter by DNA CpG methylation in vitro. Biol Chem Hoppe Seyler 377:195-201[ISI][Medline].
Rakic P (1979) Genetic and epigenetic determinants of local neuronal circuits in the mammalian central nervous system. In: The neurosciences, Fourth Study Program, pp 109-127. Cambridge, MA: MIT.
Saigal S, Lunyk O, Larke RPB, Chernesky MA (1982) The outcome in children with congenital cytomegalovirus infection. Am J Dis Child 136:896-901[Abstract].
Sanides-Kohlrausch C, Wahle P (1990) VIP and PHI immunoreactivity in olfactory centers of the adult cat. J Comp Neurol 294:325-339[ISI][Medline].
Sekerkova G, Katarova Z, Joo F, Wolff JR, Prodan S, Szabo G (1997) Visualization of beta-galactosidase by enzyme and immunohistochemistry in the olfactory bulb of transgenic mice carrying lacZ transgene. J Histochem Cytochem 45:1147-1155[Abstract/Free Full Text].
Shepherd GM, Greer CA (1990) The olfactory bulb. In: Synaptic organization of the brain (Shepherd G, ed), pp 133-169. New York: Oxford UP.
Shipley MT, McLean JH, Ennis M (1995) Olfactory system. In: The rat nervous system (Paxinos G, ed), pp 899-926. San Diego: Academic.
van den Pol AN (1985) Silver-intensified gold and peroxidase as dual ultrastructural immunolabels for pre- and postsynaptic neurotransmitters. Science 228:332-335[Abstract/Free Full Text].
van den Pol AN, Kogelman L, Ghosh P, Liljelund P, Blackstone C (1994) Developmental regulation of the hypothalamic glutamate receptor mGluR1. J Neurosci 14:3816-3834[Abstract].
Wiley CA, Nelson JA (1988) Role of human immunodeficiency virus and cytomegalovirus in AIDS encephalitis. Am J Pathol 133:73-81[Abstract].
Yang TT, Cheng L, Kain SR (1996) Optimized codon usage and chromophore mutations provide enhanced sensitivity with green fluorescent protein. Nucleic Acids Res 24:4592-4593[Abstract/Free Full Text].

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