Expression of hygR in Transgenic Mice Causes Resistance to Toxic Effects of Hygromycin B In Vivo

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Vol. 281, Issue 2, 992-997, 1997

Expression of hyg^R in Transgenic Mice Causes Resistance to Toxic Effects of Hygromycin B In Vivo¹

Jiri Aubrecht, Mary E. P. Goad², Elizabeth M. Simpson³ and Robert H. Schiestl

Department of Molecular and Cellular Toxicology, Harvard School of Public Health, 665 Huntington Ave., Boston, Massachusetts

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Aminoglycoside antibiotics are indispensable for treatment of serious bacterial infections, and despite careful attentionto dosage regimens, nephrotoxicity and ototoxicity still causeconcern. In the present study, we tested whether side effectsof aminoglycoside therapy could be limited by expression of prokaryoticgenes of antibiotic resistance in vivo. We characterized the acuteand tissue-specific toxicity of hygromycin B in transgenic micebearing the hygromycin B phosphotransferase (hyg^R) gene under control of a constitutive promoter. We characterizedthe tissue-specific expression of hyg^R mRNA and also investigated the acute toxicity of hygromycin Bin hyg^R and wild-type mice. The hyg^R mRNA reached its highest levels in brain and reached intermediatelevels in spleen, muscle, kidney, liver and testis. The lowestlevels were detected in heart and lungs. The hyg^R expression in transgenic animals caused an 89-fold increase inthe approximate lethal dose of hygromycin B compared with wild-typemice. Serum biochemical analysis of hyg^R and wild-type mice treated with lethal doses of hygromycin Bindicated liver and kidney damage measured as ALT, AST and BUN.On the morphological level, these changes led to acute tubularnephrosis in wild-type mice and acute liver damage in hyg^R mice. Our results show that constitutive expression of the bacterialhyg^R gene in transgenic mice in vivo confers resistance to hygromycinB.

	Introduction

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Hygromycin B is an aminoglycoside antibiotic produced by Streptomyces hygroscopicus (Pettinger et al., 1953) that is activeagainst both prokaryotic and eukaryotic cells. It has been shownthat in eukaryotic cells, hygromycin B acts by interfering withprotein synthesis, especially by inhibition of translocation,which is thought to be the result of its interaction with theeukaryotic ribosome displacing EF-2 from the ribosome or interferingwith the activity of EF-2 and the stabilization of peptidyl-t-RNAbound to the ribosomal acceptor site (Gonzalez et al., 1978).Toxic effects of hygromycin B in tissue culture can be preventedby expression of hyg^R (Blochlinger and Diggelmann, 1984). This enzyme adds phosphateto position 7 of the destomic acid ring of hygromycin B, whichresults in complete loss of biological activity both in vitroand in vivo (Pardo et al., 1985). Therefore, hyg^R has been widely used as a positive selective marker in the constructionof transgenic animals via ESC. The transgenic construct containinghyg^R is introduced into ESC. Then clones of ESC bearing recombinantDNA with hyg^R can be selected in medium containing hygromycin B. Although toxiceffects of hygromycin B have been studied on the cellular levelin tissue culture (see, for instance, Chen et al., 1995; Gonzalezet al., 1978; Pardo et al., 1985), we know of no previous reportson acute or tissue-specific hygromycin B toxicity in transgenicmice bearing hyg^R. For our experiments, we have used transgenic mice carrying hyg^R driven by the constitutive Pgk1 promoter (Johnson et al., 1995).These mice develop normally and do not exhibit any apparent abnormalphenotype.

The aim of our study was to investigate the influence of constitutive expression of hyg^R on the toxic effects of hygromycin B in vivo. We have examinedexpression of hyg^R mRNA in different tissues, and we have determined the approximatelethal dose of hygromycin B for hyg^R and wild-type mice. Tissue-specific changes were then evaluatedby histopathological examination and serum biochemical analysis.Our approach of using transgenic mice bearing hyg^R might contribute to better understanding of the mechanism ofaction and toxicity of aminoglycoside antibiotics.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Animals and drug treatment. Homozygous transgenic mice C57BL/6J-TgN(pPWL512hyg)1Ems carrying hyg^R (Johnson et al., 1995) and wild-type C57BL/6J were obtained fromthe Jackson Laboratory (Bar Harbor, ME). The animals were keptin specific pathogen free conditions and were supplied with standarddiet and water ad libitum. The room was held at 22°C with humidity70% and a 12-hr dark-light cycle. Animal care and experimentalprocedures were carried out in accordance with institutional guidelines.Hygromycin B was purchased from Sigma Chemical Corp (St. Louis,MO). The compound was dissolved in sterile water before application,and the solution was injected i.p.

Acute toxicity, approximate lethal dose. The approximate lethal dose of hygromycin B after single i.p. injections was determined according to Deichmann and LeBlanc(1943). This protocol significantly reduces the number of experimentalanimals, limits unnecessary suffering and complies with currentguidelines on animal studies (IARC, 1993). Two sets of 6-month-oldmale mice (22-28 g) were used for all acute toxicity experiments.The animals were treated with a single dose of hygromycin B i.p.at doses that started at 2.7 mg/kg and increased by 50% for eachconsecutive dose. Control mice were treated with the same volumeof sterile saline. Total volume injected was 0.5 ml. The healthstatus and body weights of animals were monitored daily for 10consecutive days. The lowest dose in the dose response at whichone mouse died was considered the approximate lethal dose. Deador sacrificed moribund animals were necropsied, and the organswere stored in 10% buffered neutral formalin until further analysis.The animals were checked twice a day. The maximum theoreticaltime the animals could be dead before necropsy was performed was12 hr. Because animals did not seem moribund when checked, weassume that the actual time was much less.

Histopathological examination and serum biochemical analysis. The cadavers were necropsied, and the organs were stored in 10% buffered neutral formalin. The organs were prepared as paraffin-embeddedglass slides stained with hematoxylin and eosin and were evaluatedin terms of the NTP (National Toxicology Program of NIEHS) standards.When possible, a complete cross section of each organ was evaluated(liver, spleen, gastrointestinal tract, femoral bone marrow, mandibularand mesenteric lymph nodes, kidney, brain, testes, lungs and heart).For liver, two cross sections, one of each of the two largestliver lobes, were examined. For kidneys, an entire cross section(left longitudinal, right transverse) was evaluated. Lungs hadtwo cross sections (one of each of the two largest lobes). Theentire sections on the slides (all fields) were evaluated underblind conditions for lesions and were scored (graded) on a subjectivebasis compared with control animals. The grades were as follows:1 = minimal, 2 = mild, 3 = moderate, 4 = marked and 0 = no pathologicalchanges. The preparation and evaluation of slides used the NTPcriteria and terminology (Chhabra et al., 1990).

The serum biochemistry parameters analyzed included BUN, AST and ALT. The analyses were performed at Tufts University VeterinaryMedical Diagnosis Laboratory with the chemical analyzer Hitachi747. Blood was collected from the posterior vena cava of hyg^R mice that were treated with saline 803 mg/kg and of wild-typemice administered 9 mg/kg hygromycin B i.p.

Northern blot analysis. Total RNA samples were isolated from spleen, heart, thigh muscle, lung, kidney, liver, brain and testis by guanidinium thiocyanate-phenolextraction (Chomczynski and Sacchi, 1987), separated by electrophoresisin a formaldehyde/agarose gel and transferred to a nylon HybondN+membrane (Amersham, Arlington Heights, IL) by capillary blotting.To compare loading of RNA samples we photographed the ethidiumbromide-stained gels. The blots were hybridized to a hyg^R cDNA probe (Johnson et al., 1995) that was labeled with ³²P dCTP (DuPont NEN, Boston, MA) using random oligonucleotide primers(^T7QuickPrime, Pharmacia, Piscataway, NJ). The autoradiograms wereexposed for 48 to 72 hr. The bands of hyg^R mRNA on autoradiograms and the ethidium bromide-stained 18S rRNAbands of corresponding samples were analyzed by scanning densitometrywith a BioImage (Millipore, Bedford, MA) system. To compare expressionof hyg^R mRNA, we calculated the relative IOD as total IOD of the autoradiographedband normalized to the intensity of the corresponding 18S ribosomalband visualized by ethidium bromide.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Tissue-specific expression of hyg^R. The steady-state levels of hyg^R mRNA in tissues of transgenic mice were examined by Northern blot analysis. Total RNA was isolatedfrom spleen, heart, thigh muscle, lung, kidney, liver, brain andtestes of male hyg^R-bearing transgenic and wild-type mice using guanidinium thiocyanate-phenolextraction. The RNA samples were separated by electrophoresisin a formaldehyde/agarose gel, transferred to a nylon membraneby capillary blotting and hybridized with ³²P-labeled hyg^R cDNA probe. The autoradiograms were evaluated by densitometry,and the results represent the average of three transgenic mice(fig. 1). The hyg^R mRNA reached different levels in different tissues of the hyg^R-bearing transgenic mice. No signal was detectable in wild-typemice. The highest level of hyg^R mRNA expression was detected in the brain. Mid-level expressionwas detected in skeletal muscle, testis, kidney spleen and liver,and somewhat lower levels were detected in heart and lungs.

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Fig. 1. Expression of hyg^R mRNA in mouse tissues. Total RNA was isolated and separated by electrophoresis in a formaldehyde/agarosegel, transferred to a nylon HybondN+ membrane and hybridized withlabeled hyg^R cDNA. Autoradiograms were exposed 48 to 72 hr. A) Relative levelsof expression normalized to amount of RNA loaded. Bars representsaverages ± S.E.M. B) Autoradiogram. C) Amounts of RNA loaded indifferent lanes were compared on ethidium bromide-stained gels.

Acute toxicity approximate lethal dose. The approximate lethal dose (Deichmann and LeBlanc, 1943) of hygromycin B in transgenic hyg^R-bearing as well as wild-type mice was determined as a measureof the acute toxicity. The mice were treated with single dosesof hygromycin B i.p. (2 mice per dose) that increased by 50% foreach consecutive dose. The first dose in the increasing sequenceof doses at which the mice died was considered the approximatelethal dose. The health status of animals was monitored for consecutive10 days. Hyg^R transgenic and wild-type mice tolerated a single i.p. injectionof hygromycin B without immediate toxic symptoms or distress.The approximate lethal dose of hygromycin B for wild-type micewas 6 mg/kg (table 1). Expression of hyg^R in transgenic mice caused a substantial increase in resistanceto hygromycin B. The approximate lethal dose for hyg^R animals was 535 mg/kg, which represents an 89-fold increase overthe wild-type strain. Lethal doses in both hyg^R-expressing transgenic and wild-type strains caused the same signsof decreased activity, which progressed to lethargy and death.The body weight of animals after lethal doses decreased, an effectthat was less severe at shorter survival duration after hygromycintreatment (table 1).

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TABLE 1
Acute toxicity of hygromycin B in hyg^R+/+ transgenic mice
Mice were treated i.p. with single doses of hygromycin B; controls were treated with the same volume of saline. Body weightswere measured daily for 10 days.

Serum biochemical analysis. Hyg^R mice were treated with the lethal dose of 803 mg/kg hygromycin B, and wild-type mice were treated with the lethal doseof 9 mg/kg hygromycin B. Control hyg^R mice were also treated with the nontoxic dose of 9 mg/kg. Serumsamples taken 48 hr after treatment were evaluated for the levelsof BUN, AST and ALT. Elevated BUN is associated with dehydrationand/or renal insufficiency. Elevated activities of ALT and ASTare characteristic of liver damage, particularly necrosis, cirrhosisand hepatitis. Increased AST levels are also characteristic formuscle trauma, myocardial infarction and myositis.

Administration of 9 mg/kg to wild-type mice resulted in clinically significant elevated levels of BUN, AST and ALT (table2A), which suggests renal injury and hepatocellular damage. Incontrast, the same dose given to hyg^R mice did not cause any change in those levels (table 2B). However,administration of 803 mg/kg of hygromycin B, a lethal dose tohyg^R animals, resulted in elevated levels of BUN, AST and ALT, justas the lethal dose of 9 mg/kg did in wild-type mice.

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TABLE 2
Biochemical analysis of serum after treatment of wild-type and hyg^R mice with hygromycin B
Mice were treated i.p. with single doses of hygromycin B; controls were treated with the same volume of saline. The serumsamples were taken 48 hr after treatment and frozen until analysis.The values represent averages for three animals ± S.D.

Histopathological examination. Morphological manifestations of hygromycin B tissue-specific toxicity in animals treated with lethal doses was assessed bymicroscopic analysis. Lethal doses of hygromycin B (9 mg/kg) inwild-type animals caused nephrotoxicity (table 3). These micehad tubule eosinophilia, degeneration and necrosis characterizedby cytoplasmic eosinophilia associated with necrosis, loss oftubule cellular and nuclear detail or degeneration and pyknoticnuclei and fragmentation of cells (fig. 2). These lesions aretypical of acute tubular nephrosis. Remaining tissues (liver,spleen, GI tract, femoral bone marrow, mandibular and mesentericlymph nodes, brain, testes, lungs and heart) were within normallimits (only kidney data are shown for comparison in fig. 2).The hyg^R mice treated with lethal doses of hygromycin B (803 mg/kg) hadliver damage characterized as hepatocellular fatty change, acuteinflammation and hepatocellular necrosis (table 3; fig. 3). Liverlesions in the hyg^R transgenic mice were typified by hepatocellular necrosis withnuclear pyknosis and loss of cellular detail, acute infiltrationwith small foci of neutrophils and fatty change with hepatocellularintracytoplasmic large, distinct, clear vacuoles that displacednuclei. These liver lesions are characteristic of acute liverdamage. The remaining tissues (spleen, GI tract, femoral bonemarrow, mandibular and mesenteric lymph nodes, kidney, brain,testes, lungs and heart) were within normal limits (only liverdata are shown for comparison in fig. 3).

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TABLE 3
Histopathological analysis of mouse tissues after treatment with hygromycin B
Pathological examinations were performed with five animals per dose. The tissue samples were taken and preserved in 10% bufferedneutral formalin. The values represent the average of lesion severitygrade ± S.E. (Severity grade 1 = minimal, 2 = mild, 3 = moderate,4 = marked, 0 = no pathological changes). For grading definition,see "Materials and Methods."

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Fig. 2. Kidney of wild-type and hyg^R+/+ transgenic mice after treatment with lethal doses of hygromycine B. A) Section of kidney froma wild-type mouse administered 9 mg/kg of hygromycin B has scatteredrenal tubules degeneration and necrosis in the cortex. Affectedtubules are characterized by loss of tubule cell details (arrow)and pyknosis or small nuclei (arrowheads). B) The renal corticaltubules from a transgenic hyg^R+/+ mouse treated with 803 mg/kg of hygromycin B are within normallimits (arrows). (Magnification 40×; stained with hematoxylinand eosin).

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Fig. 3. Liver of wild-type and hyg^R+/+ transgenic mice after treatment with lethal doses of hygromycin B. A) Liver from a wild-typemouse administered 9 mg/kg of hygromycin B had normal size andshape of hepatocytes (arrows) within normal limits. B) The hyg^R+/+ transgenic mice given 803 mg/kg of hygromycin B had scatteredhepatocellular necrosis characterized by pyknosis or loss of hepatocellulardetail (arrows) and hepatocellular fatty change typified by clear,eccentric round vacuoles in hepatocellular cytoplasm (arrowheads).(Magnification 40×; stained with hematoxylin and eosin).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

In the present study, we characterized the acute and tissue-specific toxicity of hygromycin B in transgenic mice bearing thehyg^R gene under control of a constitutive promoter. We characterizedthe tissue-specific expression of hyg^R mRNA, and we investigated the acute toxicity of hygromycin Bin hyg^R and wild-type mice. The hyg^R expression in transgenic animals caused an 89-fold increase inthe approximate lethal dose of hygromycin B compared with wild-typemice. Serum biochemical analysis of hyg^R and wild-type mice treated with lethal doses of hygromycin Bindicated liver and kidney damage as measured in terms of ALT,AST and BUN. On the morphological level, these changes were manifestedas acute tubular nephrosis in wild-type mice and acute liver damagein hyg^R mice. Our results show that the constitutive expression of thebacterial hyg^R gene in transgenic mice in vivo confers resistance to hygromycinB.

To evaluate hyg^R expression in vivo, we measured steady-state levels of hyg^R mRNA in different mouse tissues by Northern blot analysis. Althoughhyg^R mRNA was detected in all tissues we examined, the levels of expressionvaried. The highest level was detected in brain, and mid-levelswere measured in skeletal muscle, testis, kidney, spleen and liver.Lower levels were measured in heart and lungs. It has been reportedthat Pgk1-driven transcription of lacZ in transgenic mice is notuniform among the tissues and that the highest levels were reachedin testes and brain, that were measured mid-levels in kidney andheart followed by liver and skeletal muscle and that the lowestlevels were detected in spleen (McBurney et al., 1994). The slightlydifferent pattern of transgene expression in our study may becaused by the length of the Pgk1 promoter sequence used for hyg^R regulation, by the lack of introns and/or by differences betweenintegration sites in the genome. In case of the hyg^R mouse, the Pgk1 promoter fragment contained a promoter-specificenhancer placed directly upstream of the hyg^R gene (Johnson et al., 1995). In contrast, the lacZ constructcontained the first three exons and two introns in addition tothe Pgk1 promoter-specific enhancer (McBurney et al., 1994), whichmay have influenced expression of the transgene (Palmiter et al.,1991).

As a quantitative parameter of hygromycin B toxicity, we determined the approximate lethal dose that corresponds to the LD₅₀± 30% for most chemicals (Deichmann and LeBlanc, 1943). This protocolminimizes the number of animals needed for the assessment of acutetoxicity without unduly compromising the accuracy (Ecobichon,1992). The approximate lethal dose in wild-type mice for hygromycinB after i.p. application in our experiments was 6 mg/kg. Thisvalue is identical to the LD₅₀ estimate after i.v. applicationusing conventional methods (Berdy, 1980), which indicates thatthe approximate lethal dose is an appropriate parameter for evaluatingthe acute toxicity of hygromycin B in vivo. Transgenic hyg^R positive mice showed a dramatic 89-fold increase in the approximatelethal dose over the wild-type strain. This suggests that thelevel of Hyg^R enzyme present in the cells of the transgenic mice effectivelydecreased hygromycin B toxicity in vivo.

To characterize the organ targets of hygromycin B toxicity in wild-type and hyg^R transgenic mouse, we performed biochemical analysis and histopathologicalevaluation of mice treated with lethal doses of hygromycin B.The kidney damage was characterized as an alteration in BUN levels,and liver damage was evaluated as a change of ALT and AST activities.Serum biochemical analysis of both wild-type and hyg^R mice treated with lethal doses of hygromycin B (9 mg/kg and 803mg/kg, respectively) revealed renal injury characterized as increasedlevels of BUN and liver damage characterized as an increase inALT and AST enzymatic activities. Morphological correlates tothe serum biochemical results were characterized using histopathologicalanalysis. The wild-type mice treated with lethal doses of hygromycinB showed histological signs of nephrotoxicity identified as tubuleeosinophilia, degeneration and necrosis. In contrast, the transgenichyg^R transgenic mice treated with toxic doses of hygromycin B showedhistopathological signs of liver damage characterized as hepatocellularfatty changes, acute inflammation and hepatocellular necrosis.Although the serum biochemical analysis and histopathologicalfindings in wild-type and hyg^R mice differ, the liver and kidney seem to be the targets of hygromycinB toxicity in both mouse strains. The weak correlation betweenbiochemical markers and histopathological findings has been reportedin other instances, so organ-specific damage must be characterizedby using more than one parameter (Baum et al., 1975; Herrera,1993). It seems that in hyg^R mice, the lethal doses of hygromycin B overloaded the metaboliccapacities of Hyg^R enzyme to inactivate the drug. The absence of hepatic or renalhistopathological manifestation of hygromycin B toxicity in wild-typeanimals or hyg^R mice, respectively, may be explained by different availabilityof active hygromycin B molecules in liver and kidney.

Pathological manifestations of renal toxicity associated with aminoglycoside therapy consist largely of acute tubular lesionsand necrosis resulting in kidney failure (Laurent et al., 1990;Tulkens, 1989). This pathological pattern of tissue injury correlateswith the pharmacokinetics and disposition of aminoglycosides.After application, the aminoglycosides are excreted unchangedthrough the kidneys (Sande and Mandell, 1985), where a portionof the dose is reabsorbed and cumulated in the tubular cells ofthe renal cortex (Giuliano et al., 1986; Kuhar et al., 1979).The association of aminoglycosides with negatively charged phospholipidsand their accumulation in the lysosomes of tubular cells leadsto phospholipidosis by inhibition of lysosomal phospholipases(Laurent et al., 1982), which may trigger necrosis (Laurent etal., 1990). On the other hand, it has also been shown on the cellularlevel that hygromycin B interferes with protein synthesis, especiallyby inhibition of translocation (Gonzalez et al., 1978). Our resultsindicate that compared with aminoglycosides used in therapy, hygromycinB caused not only clinically similar kidney damage but also livertoxicity. The exact molecular mechanism of hygromycin B toxicityand the degree of its possible interaction with phospholipidsand/or protein synthesis in vivo remain to be elucidated.

Aminoglycoside antibiotics are indispensable for treatment of serious infectious diseases. Despite careful attention to dosageregimens designed to achieve targeted levels in the serum, theirtoxicity still causes concern (Lortholary et al., 1995). Althoughhygromycin B is not used for treatment of human patients, ourresults clearly show that its toxicity can be prevented by expressionof hyg^R in vivo. The general approach of using transgenic animals withspecific changes in drug metabolism pathways can contribute toour understanding of the mode of action and toxicity of drugs.This could ultimately lead to improvement of drug design and treatmentregimens.

	Acknowledgments

We thank the members of the Schiestl laboratory for discussions and comments on the manuscript. We thank Kristie Wetzel forproviding histology support services and Charles P. Lerner forbreeding mice.

	Footnotes

Accepted for publication January 22, 1997.

Received for publication August 12, 1996.

¹ This work was supported by grant No. 1RO1ES07694 from the National Institutes of Health to R.H.S., grant No. MCB-9513537 fromthe National Science Foundation to E.M.S. and NIH Cancer CoreGrant CA34196 at Jackson Laboratory.

² Department of Veterinary Pathology, School of Veterinary Medicine, Louisiana State University, Baton Rouge, LA 70803.

³ The Jackson Laboratory, 600 Main Street, Bar Harbor, ME 04609.

Send reprint requests to: Robert H. Schiestl, Department of Molecular and Cellular Toxicology, Harvard School of Public Health, 665 Huntington Ave, Boston, MA 02115.

	Abbreviations

ALT, alanine aminotransferase; AST, aspartate aminotransferase; BUN, blood urea nitrogen; ESC, embryonic stem cells; hyg^R, hygromycin B phosphotransferase; IOD, integrated optical density; LD₅₀, median lethal dose.

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Expression of hygR in Transgenic Mice Causes Resistance to Toxic Effects of Hygromycin B In Vivo1

Expression of hyg^R in Transgenic Mice Causes Resistance to Toxic Effects of Hygromycin B In Vivo¹