EcRexpressionintheprothoracicotropic hormone-
producing neurosecretorycellsoftheBombyxmori brain
An indication ofthe master cellsof insect metamorphosis
Monwar Hossain
1
, Sakiko Shimizu
2
, Haruhiko Fujiwara
3
, Sho Sakurai
1,2
and Masafumi Iwami
1,2
1 Division of Life Sciences, Graduate School of Natural Science and Technology, Kanazawa University, Japan
2 Division of Biological Science, Graduate School of Natural Science and Technology, Kanazawa University, Japan
3 Department of Integrated Biosciences, Graduate School of Frontier Sciences, The University of Tokyo, Kashiwa, Japan
The insect brain is the center of developmental control.
In thebrainofthe silkworm Bombyx mori, two pairs
of lateral neurosecretorycells (LNCs) produce the
prothoracicotropic hormone (PTTH) [1,2]. The peptide
PTTH stimulates the prothoracic glands to synthesize
and release ecdysone [3]. The active form of ecdysone,
20-hydroxyecdysone (20E), controls many physiologi-
cal and developmental processes of insect molting and
metamorphosis [4]. Beside PTTH, thebrain produces
many neurosecretory hormones that orchestrate devel-
opmental processes. It is also the target organ of 20E,
effecting dynamic morphological changes and rear-
rangement ofthe neural network during processes such
as the formation ofthe optic lobe and mushroom body
differentiation during metamorphosis [5,6]. Hence, the
analysis of 20E-induced gene expressioninthebrain is
of critical importance in understanding insect develop-
ment.
The 20E signal is mediated intrinsically through
binding with its heterodimeric nuclear receptor consist-
ing ofthe ecdysone receptor (EcR) and ultraspiracle
(USP) [7,8]. The 20E–receptor complex directly induces
several early genes and the products of these genes
activate late effector genes that control stage- and
tissue-specific developmental responses to 20E [9]. Two
EcR isoforms, EcR-A and EcR-B1, and two USP iso-
forms, usp-1 and usp-2, which have been identified in
Bombyx [10–13], are involved in specific responses to
Keywords
Bombyx mori; brain; ecdysone receptor;
metamorphosis; prothoracicotropic
hormone-producing neurosecretory cell
Correspondence
M. Iwami, Division of Life Sciences,
Graduate School of Natural Science and
Technology, Kanazawa University,
Kanazawa 920-1192, Japan
Fax: +81 76 2646251
Tel: +81 76 2646255
E-mail: masafumi@kenroku.kanazawa-u.ac.jp
(Received 18 May 2006, revised 22 June
2006, accepted 26 June 2006)
doi:10.1111/j.1742-4658.2006.05398.x
The steroid hormone 20-hydroxyecdysone (20E) initiates insect molting and
metamorphosis through binding with a heterodimer of two nuclear recep-
tors, the ecdysone receptor (EcR) and ultraspiracle (USP). Expression of
the specific isoforms EcR-A and EcR-B1 governs steroid-induced responses
in the developing cellsofthe silkworm Bombyx mori. Here, analysis of
EcR-A and EcR-B1 expression during larval-pupal development showed
that both genes were up-regulated by 20E inthe B. mori brain. Whole-
mount in situ hybridization and immunohistochemistry revealed that
EcR-A and EcR-B1 mRNAs and proteins were exclusively located in two
pairs of lateral neurosecretorycellsinthe larval brain known as the pro-
thoracicotropic hormone (PTTH)- producing cells (PTPCs). Inthe pupal
brain, EcR-A and EcR-B1 expression was detected in tritocerebral cells and
optic lobe cellsin addition to PTPCs. As PTTH controls ecdysone secre-
tion by the prothoracic gland, these results indicate that 20E-responsive
PTPCs are the master cellsof insect metamorphosis.
Abbreviations
20E, 20-hydroxyecdysone; EcR, ecdysone receptor; LNC, lateral neurosecretory cell; MEF2, myocyte enhancer factor 2; OLC, optic lobe cell;
NaCl ⁄ P
i
⁄ Tween, phosphate buffered saline containing Tween; PTPC, PTTH-producing neurosecretory cell; PTTH, prothoracicotropic
hormone; TCC, tritocerebral cell; USP, ultraspiracle.
FEBS Journal 273 (2006) 3861–3868 ª 2006 The Authors Journal compilation ª 2006 FEBS 3861
20E. EcR-A expression regulates neuronal maturation,
while EcR-B1 expression controls neuronal regression
both in Drosophila melanogaster [14,15] and Manduca
sexta [16]. Mutational analysis ofEcR isoforms in
Drosophila identified several different lethal phases,
including developmental arrest late in embryogenesis,
failure of pupariation [17,18], and disruption of neur-
onal remodeling [18]. Although the effect of ecdysone
on neurons ofthe central nervous system has been
extensively studied in Drosophila and Manduca, little
information is available on the role ofEcR expression
in the brain. Inthe present study, we examined EcR-A
and EcR-B1 expressionintheBombyxbrain and
demonstrate stage- and cell-specific expressionof EcR
isoforms, which is especially prominent in PTTH-
producing cells (PTPCs). These results provide an
insight into ecdysone receptor function inthe brain
during larval-pupal-adult development.
Results
Expression of EcR-A and EcR-B1 inthe Bombyx
brain
Day-2 fifth instar B. mori larvae were injected with
1 lg 20E (+20E) or Ringer’s solution ()20E), and
RNA was extracted from the brains 2 h after the injec-
tions. RT-PCR revealed that both EcR-A and EcR-B1
were weakly expressed inthe absence of 20E, and
that 20E up-regulated theexpressionof both genes
(Fig. 1A). EcR-A was shown to be expressed at a
slightly higher level than EcR-B1 following induction
by 20E. No transcript was amplified after 25 cycles of
RT-PCR for both +20E and )20E samples. Expres-
sion ofthe control housekeeping gene RpL32 showed
no difference between +20E and )20E samples after
25 and 35 cycles of RT-PCR.
To examine spatial expressionofEcR isoforms,
we carried out RT-PCR on RNA purified from the
anterior and the posterior sections of B. mori brains
(Fig. 1B). Intense EcR-A expression was observed
exclusively inthe anterior part while no expression
was detected inthe posterior part after 35 cycles of
RT-PCR (Fig. 1C). Strong EcR-B1 expression was also
detected inthe anterior part ofthebrain and weaker
expression was detected inthe posterior section, indi-
cating that both genes exhibit a spatial-specific pattern
of expression. RpL32 expression did not differ between
the two parts ofthe brain.
Cell-specific expressionofEcR isoforms as
revealed by in situ hybridization
The spatial specificity of EcR-A and EcR-B1 expres-
sion was also determined by whole-mount in situ
hybridization of larval and pupal brains using EcR iso-
form-specific probes. EcR-A expression was detected
exclusively in two pairs of lateral neurosecretory cells
(LNCs) in day-2 (Fig. 2A) and day-7 (Fig. 2C) fifth
instar larval brains. The location ofthe EcR-A-positive
cells was assumed to be the same as that of PTTH-
producing cells (PTPCs), as shown in Fig. 2E. To con-
firm this, we performed in situ hybridization using a
mixture of EcR-A and PTTH probes. The hybridiza-
tion signal was again detected exclusively inthe two
pairs of LNCs (Fig. 2G), indicating that EcR-A and
PTTH mRNAs were colocalized in PTPCs ofthe lar-
val brain. EcR-B1 expression was also detected exclu-
sively inthe same LNCs in day-2 (Fig. 2B) and day-7
(Fig. 2D) fifth instar larval brains, while EcR-B1 and
PTTH expression was shown to colocalize in PTPCs
of the larval brain (Fig. 2H).
In the pupal brain, EcR-A expression was observed
in PTPCs (Fig. 2I,L) and in several tritocerebral cells
(TCCs) (Fig. 2K) and optic lobe cells (OLCs) (Fig. 2J).
EcR-B1 expression was similarly detected in PTPCs
(Fig. 2F), TCCs, and OLCs (Fig. 3E) but at a lower
level than EcR-A. In addition to the brain, faint
EcR-A expression was detected inthe subesophagal
ganglion (Fig. 2K). Both EcR isoforms are therefore
A
B
C
Fig. 1. EcR-A and EcR-B1 are induced by 20E and are predominantly expressed inthe anterior of day-2 fifth instar larval brains. (A) RT-PCR
analysis of EcR-A and EcR-B1 expression following injection of 20E (+20E) or Ringer’s solution ()20E). The number of PCR cycles is indica-
ted above the panel. The housekeeping gene RpL32 was used as a control. (B) Total RNA was extracted either from the anterior (A) or pos-
terior (P) part ofthe brains and analyzed by RT-PCR to assess the spatial distribution of gene expression. (C) RT-PCR analysis of EcR
expression using RNA from the anterior (A) and posterior (P) part ofthe brains. The number of PCR cycles is indicated above the panel.
EcR expressionin PTTH cellsofBombyxmoribrain M. Hossain et al.
3862 FEBS Journal 273 (2006) 3861–3868 ª 2006 The Authors Journal compilation ª 2006 FEBS
expressed exclusively in PTPCs at the larval stage and
in PTPCs, TCCs, and OLCs inthe pupal stage of
B. mori development.
Immunohistochemical confirmation of EcR-A and
EcR-B1 cell-specific expression
To confirm thein situ hybridization results, we
performed double-labeled immunohistochemistry with
anti-EcR-A and anti-EcR-B1 sera, and anti-PTTH IgG
on the brains of day-2 and day-7 fifth instar larvae
and day-2 pupae. EcR-A and PTTH expression was
detected exclusively in two pairs of LNCs in day-2 fifth
instar larvae (Fig. 3A, left). The merged image shows
that EcR-A and PTTH expression colocalizes in
PTPCs. This colocalization was also observed in day-7
larval and day-2 pupal brains (Fig. 3B,C, left). The
same results were obtained for EcR-B1 (Fig. 3A–C,
right), confirming that both isoforms are colocalized in
PTPCs inthe brain.
In the pupal brain, EcR-A and EcR-B1 expression
was observed in TCCs and weakly in OLCs in addi-
tion to PTPCs (Fig. 3D,E, also Fig. 2I,J). It is note-
worthy that EcR-B1 fluorescence was strongest just
beneath the cell membrane of TCCs (Fig. 3F) and
was weaker inthe axons, while EcR-A fluorescence
was more diffuse throughout the cytoplasm (Fig. 3D,
also Fig. 3A), indicating that the distribution of the
two isoforms differed slightly. EcR-A and EcR-B1
expression was also detected inthe subesophagal gan-
glion (Fig. 3D,E).
Discussion
In the present study, we have shown for the first
time that EcR-A and EcR-B1 are up-regulated by 20E
AB
DC
EF
HG
I
J
K
L
Fig. 2. Localization of EcR-A, EcR-B1 and
PTTH mRNAs by whole-mount in situ
hybridization. EcR-A and EcR-B1 mRNA was
detected in day-2 (A,B) and day-7 (C,D) fifth
instar larval brains and day-2 pupal brains
(F,I). For fifth instar day-2 specimens, brains
were dissected 2 h after 20E injection.
PTTH mRNA was detected in day-2 fifth
instar larval brains (E). (G) EcR-A and PTTH
as well as (H) EcR-B1and PTTH probes
were used simultaneously for hybridization
of day-2 larval brains. (A–E,G,H) show the
anterior portion ofthe larval brain. EcR-A
expression inthe pupal brain (I) is magnified
in panels J–L, where OLCs (J, white
arrows), TCCs (K, white arrows) and PTPCs
(L, white arrows) are shown in green, blue,
and black boxes, respectively. The blue
arrows in K indicate faint signals inthe sub-
esophagal ganglion. Scale bar ¼ 100 lm.
M. Hossain et al. EcRexpressionin PTTH cellsofBombyxmori brain
FEBS Journal 273 (2006) 3861–3868 ª 2006 The Authors Journal compilation ª 2006 FEBS 3863
exclusively in PTPCs inthe B. mori larval brain. The
spatial specificity of EcR-A and EcR-B1 expression
was determined by in situ hybridization and confirmed
by immunohistochemistry using EcR isoform-specific
antibodies.
Expression of EcR-A and EcR-B1 in PTPCs has not
been reported previously. Recently, Vafopoulou et al.
[19] used immunohistochemistry to demonstrate EcR
expression inthe medial neurosecretorycellsof Rhodn-
ius prolixus. The postembryonic development of
Rhodnius and Bombyx is strikingly different. Unfed
Rhodnius larvae exist in an arrested developmental
state caused by an ecdysteroid deficiency [20], which is
immediately met by the consumption of a blood meal,
thus initiating development. No such phenomenon
exists inBombyx larvae, and it is possible that the
difference in 20E-responsive cells between the two
insects reflects the different developmental systems.
Our study indicates that theexpression level of EcR-
A is slightly higher than that of EcR-B1, as previously
observed during the neuronal maturation of Drosophila
and Manduca [16]. The developmental function of
EcR-A is distinct from those mediated by the EcR-B1
and EcR-B2 isoforms in Drosophila.AnEcR-A mutant
is arrested during early to mid-pupal development,
indicating that EcR-A is required for the formation of
the basic pupal body plan prior to the differentiation
of most adult structures [15]. By contrast, an EcR-B1
mutant is lethal at the first and second larval molts
[18] and fails to undergo pupariation [17].
PTPCs are the only cells to express EcR isoforms in
the Bombyx larval brain, and these cells also express
A
B
C
D
F
E
Fig. 3. Immunohistochemical localization of
EcR-A, EcR-B1, and PTTH. (A) Day-2 larval,
(B) day-7 larval and (C) day-2 pupal brains.
For fifth instar day-2 specimens, brains were
dissected 6 h after 20E injection. Anti-EcR-A,
anti-EcR-B1, and anti-PTTH were used as
primary antibodies. A FITC-conjugated anti-
rabbit secondary antibody was used to
detect EcR-A or EcR-B1, and a Texas-red
conjugated anti-mouse secondary antibody
was used to detect PTTH. The middle panel
(A–C) shows a merged (yellow) image of
the upper (green, EcR-A or EcR-B1) and
lower (red, PTTH) panels. (D) EcR-A and (E)
EcR-B1 expressionin day-2 pupal brains.
White arrows in (D) and (E) indicate the
EcR-A- and EcR-B1-producing cellsin the
tritocerebral region ofthe pupal brain,
respectively. Red arrows indicate the EcR-A-
or EcR-B1-producing cellsinthe subesopha-
gal ganglion, respectively. A magnified
image ofthe red box in (E) is shown in (F),
where EcR-B1 expression is indicated by
white arrows. Scale bar ¼ 100 lm.
EcR expressionin PTTH cellsofBombyxmoribrain M. Hossain et al.
3864 FEBS Journal 273 (2006) 3861–3868 ª 2006 The Authors Journal compilation ª 2006 FEBS
usp isoforms (MDM Hossain & M Iwami, unpub-
lished data). As the 20E signal is transduced via the
EcR–USP complex, it can be concluded that PTPCs
are the only cells to respond to 20E at the transcrip-
tional level, and these cells therefore play important
roles in 20E-dependent larval-pupal metamorphosis.
PTTH controls the hemolymph 20E level by stimula-
ting ecdysone synthesis and coordinating its release
from the prothoracic glands. EcR-A and EcR-B1
expression inthe PTPCs suggests that 20E modulates
PTTH expression through a feedback loop. Beside its
prothoracicotropic effect, PTTH may act as a growth
factor as it shares a common ancestor with the verteb-
rate growth factor superfamily peptides such as nerve
growth factor, transforming growth factor, and plate-
let-derived growth factor [21]. It also enhances the syn-
thesis of several short-lived proteins that mediate a
variety of extracellular signals [22,23]. Despite the first
demonstration of PTTH almost three decades ago in
LNCs in Manduca [24] and later inBombyx [1,2],
the molecular mechanisms of PTTH production and
release are still at an early level of understanding,
although these are of critical importance in insect
developmental control [25].
Since the work of Truman [26], it has been believed
that PTTH release is controlled by a circadian clock in
the brain [27–29]. The close association between clock
cells and PTPCs inthebrain protocerebral region is
seen inthe three divergent genera Rhodnius, Dro-
sophila, and Bombyx, suggesting that there are routes
of communication between these two cell populations
[30,31]. The association with clock cells and the
responsiveness of PTPCs for ecdysteroidogenesis sug-
gests that 20E influences PTTH release from PTPCs
through neurons that provide input to clock cells
[31,32]. The PTTH titer inBombyx larval hemolymph
is, however, not exclusively controlled by photoperiod
and ⁄ or circadian clock mechanisms [27,28], as protho-
racicostatic hormones have been shown to influence
ecdysteroidogenesis and ecdysteroid release from the
PTTH-stimulated prothoracic gland [33,34]. At the
transcriptional level, Bombyx PTTH is regulated by
trans-regulatory factors such as myocyte enhancer fac-
tor 2 (MEF2) [32]. Inthe brain, MEF2 is expressed at
an elevated level in PTPCs and corazonin-like immu-
noreactive-LNCs. Over-expression of MEF2 increases
PTTH expressioninBombyxbrain [32], while up-regu-
lation of MEF2 by 20E was reported in adult Dro-
sophila myoblasts [35]. An emerging hypothesis is that
MEF2 is regulated by 20E, which in turn modulates
PTTH expression.
In addition to PTPCs, EcR-A and EcR-B1 expres-
sion was detected inthe tritocerebrum and the optic
lobe of day-2 pupae: a crucial stage for the morpholo-
gical and neurological reorganization ofthe brain. 20E
induces differentiation ofthe optic lobe and adult eye
in Manduca [5,36], while EcR is expressed during the
puparium stage inthe optic lobe of Drosophila [16]. In
the present study, EcRexpressionin B. mori OLCs is
consistent with these findings. Inthe tritocerebrum, the
number and position of EcR-A-producing cells differed
from EcR-B1-producing cells. The intracellular local-
ization of EcR-A was also distinct from that of
EcR-B1: EcR-A was localized inthe cytoplasm while
EcR-B1 was beneath or close to the cell membrane of
PTPCs and TCCs. The intracellular distribution of
EcR-B1 could indicate a nongenomic role for 20E in
these cells [37].
The present results clearly show that EcR isoform
expression inthebrain is exclusive to the PTPCs until
pupation. This indicates that PTPCs are the master
cells during larval-pupal metamorphosis and that they
control ecdysteroidgenesis. At the pupal stage, the
number ofcells expressing EcR isoforms increases to
include TCCs and OLCs. This unique expression pro-
file indicates the importance ofEcR isoform expression
in TCCs and OLCs during larval-pupal metamorpho-
sis, although the roles ofthe individual isoforms in
these cells remain to be elucidated.
Experimental procedures
Animals and hormones
B. mori eggs of a racial hybrid, Kinshu · Showa were
obtained from Ueda Sanshu (Ueda, Japan), and larvae
were reared on an artificial diet (Silkmate II, Nihon Nou-
san Kogyo, Yokohama, Japan) under a 12 h light ⁄ 12 h
dark photoperiod at 25 ± 1 °C [38]. Ages were counted in
days, consisting of a photophase followed by a scotophase.
Fifth instar day-2 and day-7 larvae and day-2 pupae were
studied. 20E (Sigma, St. Louis, MO, USA) was dissolved in
ethanol and its concentration was determined spectrophoto-
metrically at 243 nm (e
EtOH
¼ 12 300). An aliquot of the
stock solution was evaporated and dissolved in insect Ring-
er’s solution (130 mm NaCl, 4.7 mm KCl, 1.9 mm CaCl
2
).
RNA isolation and semiquantitative RT-PCR
Total RNA was isolated from whole brains 2 h after the
injection of 20E (1 lg per larva) (+20E) or insect Ringer’s
solution ()20E) as a control. To determine the region of
expression inthe brain, total RNA was isolated from the
anterior and posterior sections of brains. RNA was purified
by the acid guanidinium-thiocyanate ⁄ phenol ⁄ chloroform
method [39] with minor modifications [40].
M. Hossain et al. EcRexpressionin PTTH cellsofBombyxmori brain
FEBS Journal 273 (2006) 3861–3868 ª 2006 The Authors Journal compilation ª 2006 FEBS 3865
One microgram total RNA was reverse-transcribed in a
20 lL reaction using 100 U ReverTra Ace (Toyobo, Osaka,
Japan) and 5 pmol oligo(dT)
12)18
at 42 °C for 1 h accord-
ing to the manufacturer’s instructions. After reverse tran-
scription, the reaction was stopped by heating the solution
at 99 °C for 5 min, and the cDNA solution was diluted
five-fold with water. PCR primers were designed according
to the nucleotide sequences: EcR-A 5¢-TGGAGCTGAAA
CACGAGGTGGC-3¢ and 5¢-TCCCATTAGGGCTGTAC
GGACC-3¢, EcR-B1 5¢-ATAACGGTGGCTTCCCGCTG
CG-3¢ and 5¢-CGGTGTTGTGGGAGGCATTGGTA-3¢,
and RpL32 5¢-GAGGACGAAGAGATTTATCAGGCA-3¢
and 5¢-CGAAGAGACACCATGAGCGAT-3¢. PCR was
carried out in a 10 lL volume containing 10 mm Tris ⁄ HCl
(pH 8.8), 50 mm KCl, 1.5 mm MgCl
2
, 0.08% (v ⁄ v) Noni-
det P40, 0.2 mm each dNTPs, 0.5 mm each primer, 0.25 U
Taq DNA polymerase (Fermentas, Burlington, Ontario,
Canada), and 1 lL synthesized cDNA. The reaction was
subjected to 25 or 35 cycles of amplification in a thermo-
cycler (GeneAmp PCR System 9700, Applied Biosystems,
Foster City, CA, USA) using a thermal cycle (94 °C, 30 s;
60 °C, 30 s; 72 °C, 30 s). PCR products were separated on
a 1.5% (w ⁄ v) agarose gel and visualized by ethidium bro-
mide staining. There was no amplification without reverse
transcriptase even at 35 cycles of PCR (data not shown),
indicating the specificity of EcR-A and EcR-B1 mRNA
amplification.
In situ hybridization
Whole-mount in situ hybridization of brains was performed
as described previously [41]. After dissecting, brains were
washed with 10 mm phosphate buffered saline, pH 7.4
NaCl ⁄ P
i
⁄ 0.05% Tween20 and fixed in 85% (v ⁄ v) ethanol,
4% (w ⁄ v) formaldehyde, and 5% (v ⁄ v) acetic acid on ice
for 40 min. The brains were then incubated in a solution of
NaCl ⁄ P
i
containing 15% (w ⁄ v) sucrose at 4 °C for 15–20 h.
After washing with NaCl ⁄ Pi ⁄ 0.05% Tween20, the brains
were treated with proteinase K (0.05 mgÆmL
)1
in NaCl ⁄
Pi ⁄ 0.05% Tween20) at 37 °C for 40 min, and fixed again
with 3% (w ⁄ v) paraformaldehyde in NaCl ⁄ P
i
at room tem-
perature for 20 min. The brains were washed three times
with NaCl ⁄ P
i
⁄ 0.05% Tween20 and hybridized with 60 ng
EcR-A probe (5¢-TCCCATTAGGGCTGTACGGACC-3¢)
or EcR-B1 probe (5¢-CGGTGTTGTGGGAGGCATTG
GTA-3¢) and ⁄ or PTTH probe (5¢-GTACACAAACACGCC
ACGCTGACG-3¢)3¢-labeled with digoxigenin using a
Dig-labeled kit (Roche Diagnostics, Mannheim, Germany).
Hybridization was carried out at 37 °C for 20–48 h in a
100 lL hybridization solution [50% (v ⁄ v) formamide,
5· standard sodium citrate (NaCl ⁄ Cit; 0.15 m NaCl,
0.015 m sodium citrate), 5% (w ⁄ v) dextran sulphate]. After
sequential washing with 50% (v ⁄ v) formamide, 5 · NaCl ⁄
Cit and NaCl ⁄ P
i
⁄ 0.05% Tween20 at room temperature, the
brains were treated with 5% (v ⁄ v) sheep serum
(Rockland, Gilbertsville, PA, USA) at 4 °C for 15–20 h,
followed by a 2 h incubation with a 1 : 500 diluted alkaline
phosphatase conjugated anti-digoxigenin IgG (Roche
Diagnostics) at room temperature. Color development
was performed with 4-nitroblue-tetrazolium chloride
(336.4 lgÆmL
)1
) and 5-bromo-4-chloro-3-indolyl phos-
phate (175 lgÆmL
)1
) inthe presence of 1 mm levamisole, a
potent inhibitor of endogenous alkali phosphatases. After
dehydration with ethanol, the brains were clarified with
methyl salicylate and observed with a microscope (BX-50F,
Olympus, Tokyo, Japan). Negative controls omitted the
labeled probes, and no signal was detected (data not
shown).
Anti-peptide serum for BombyxEcR isoforms
An EcR-A specific peptide [H
2
N-GQVKAEPGVSHN
GHP(15–29)C-COOH] [13] (Accession no D87118) and an
EcR-B1 specific peptide [H
2
N-CPLPMPPTTPKSENES
MSSG(94–112)-COOH] [12] (Accession no D43943) were
synthesized, HPLC purified, and used to immunize rabbits
(Sawady Technology, Tokyo, Japan). Handling of rabbits
was performed according to regulation and guidelines of
the local authority. The anti-peptide serum titers for EcR-A
and EcR-B1, determined using an enzyme-linked immuno-
sorbent assay, were 4700 and 119 700, respectively.
Immunohistochemistry
Double-labeled fluorescent immunohistochemistry was used
to detect EcR-A, EcR-B1, and PTTH expression. Brains
were washed with NaCl ⁄ P
i
, fixed in Bouin’s solution over-
night, then washed with 70% (v ⁄ v) ethanol. The brains
were then soaked in 0.1% (w ⁄ v) sodium deoxycholate and
2% (v ⁄ v) Tween20 in NaCl ⁄ P
i
at 4 °C for 4 days to facili-
tate the penetration of antibodies through thebrain sheath
[2]. The pretreated brains were incubated with rabbit anti-
Bombyx EcR-A serum (1 : 200) or anti-Bombyx EcR-B1
serum (1 : 300) and mouse anti-Bombyx PTTH monoclonal
IgG (1 : 100) [2] overnight. The brains were then incubated
simultaneously at 4 °C overnight with the secondary anti-
bodies, mouse anti-rabbit IgG conjugated with fluorescein
isothiocyanate (Cappel, Aurora, OH, USA) at a dilution of
1 : 400 for EcR-A and EcR-B1, and goat anti-mouse IgG
conjugated with Texas-Red (Cappel) at a dilution of 1 : 400
for PTTH. The brains were washed with NaCl ⁄
P
i
⁄ 0.05% Tween20 and clarified with methyl salicylate.
Fluorescence was detected using a fluorescence microscope
(BX-50F, Olympus) using NIBA filters for fluorescein isoth-
iocyanate and WIY filters for Texas-Red. Negative controls
replaced the primary antibodies with NaCl ⁄ P
i
⁄ 0.05%
Tween20 (data not shown). The absence of detectable flo-
rescence in these controls demonstrated the specificity of
the reaction. Images were processed with Adobe Photoshop
(Adobe Systems Inc, San Jose, CA, USA).
EcR expressionin PTTH cellsofBombyxmoribrain M. Hossain et al.
3866 FEBS Journal 273 (2006) 3861–3868 ª 2006 The Authors Journal compilation ª 2006 FEBS
Acknowledgements
We are grateful to Dr A. Mizoguchi for the gift of
the anti-PTTH antibody. This work was supported by
Grants-in-Aid for Scientific Research (15580039 and
18380040) from the Japan Society for the Promotion
of Science.
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. EcR expression in the prothoracicotropic hormone-
producing neurosecretory cells of the Bombyx mori brain
An indication of the master cells of insect. available on the role of EcR expression
in the brain. In the present study, we examined EcR- A
and EcR- B1 expression in the Bombyx brain and
demonstrate stage-