Biểu hiện gen?

[bionhien]

Em đang gặp vấn đề biểu hiện
Em làm nhiều lần mà cũng ko có kết quả khả quan. Các bước của em: nuôi lượng nhỏ- nuôi lượng lớn- cảm ứng IPTG- thu tế bào - ly tâm thu tủa- điện di.
Anh chị nào có kinh nghiệm làm về biểu hiện thì giúp cho em với.
Em cám ơn nhiều

 

[Nguyễn Duy Hưng]

Em có làm thao tác tinh sạch nào sau ly tâm thu tế bào ko.

 

[bionhien]

dạ ko anh, em chỉ ly tâm thu tế bào-sau đó để tủ -200C, rồi đem điện di thôi

 

[Nguyễn Duy Hưng]

Em làm với E. coli à? Với deep freeze - thaw như vậy chắc cũng đủ phá vỡ tế bào gùi. Em thử làm thêm 1 bước cell lysis xem sao. Em có thể post hình của các gel em thu đc ko.

 

[bionhien]

em chào anh
thật sự em ko biet post hình ảnh lên,anh cho em địa chỉ email của anh rồi em gởi qua cho anh,
em cám ơn anh nhé

 

[Nguyễn Duy Hưng]

Em send thử qua email này duyhung1984@yahoo.com

 

[Nguyễn Duy Hưng]

Em gửi ảnh mà ko chú thích các land, MW marker và cả MW của protein mà em muốn biểu hiện thì anh chịu.
Anh chỉ nhận xét là protein trong mẫu của em hơi nhiều, em nên pha loãng thêm hay tinh sạch 1 phần trước khi loading lên gel
Anh post hình của em lên đây cho mọi ng khác có thể xem đc

 

[bionhien]

nhưng pha loãng hay tinh sạch thì làm cách nào thế anh, anh giúp em với

 

[Nguyễn Duy Hưng]

Em phải định lượng protein trong mẫu của em sau đó pha loãng đến khoảng 100 - 500 ug/ml trước khi load vài gel
Tinh sạch thì đơn giản nhất là lọc gel. Nhưng sẽ khó khăn cho em khi xác định fraction nào có protein của em nếu em ko có assay để định tính nó.

 

[Cao Xuân Hiếu]

Có băng biểu hiện trên gel rồi, có lẽ nằm ở inclussion body.

Làm theo hướng dẫn sau thì sẽ chuẩn ko cần chỉnh:

1. Nuôi vk qua đêm trong mt có kháng sinh thích hợp (V=5mL). Tốt nhất là bắt đầu từ 1 khuẩn lạc trên đĩa thạch. Dùng 2 culture là 1) sample = vk mang recombinant plasmid; 2) control = vk cùng dòng (genetic background) mang empty plasmid. Nếu ko có thì lấy vk cùng genetic background là OK.

2. Đo OD của 02 culture ovn. Bắt đầu 03 môi trường mới (V=5mL) có kháng sinh (2x sample + 01 control). Cho vào môi trường 1 thể tích nhất định của culture ovn sao cho nồng độ OD cuối là 0.05 OD unit/mL

3. Theo dõi OD660 cho đến khi OD đạt 0.4 thì bỏ IPTG vào 1 sample và 1 control.

4. Chờ 2 giờ sau thì do lại OD660 và thu 01mL của 03 culture: 1) sample + IPTG, 2) sample - IPTG, 3) control + IPTG

5. Ly tâm thu cặn tế bào 6000 rpm, 8 min. Cất vào -20oC cho qua đêm.

6. Hòa cặn tế bào trong dung dịch 2x SDS sample buffer với thể tích tương ứng sao cho nồng độ cuối là 0.01OD unit/ ul (microlitter). Dựa vào giá trị OD đo sau khi cảm ứng 2h.

7. Heat eppendorf ở 98oC trong 10min. Spin down.

8. Load lên gel 05 ul trong mỗi giếng theo thứ tự 1) Protein ladder (marker), 2) control + IPTG, 3) sample - IPTG, 4) sample + IPTG

9 Nhuộm coomassie blue rồi scan gửi lên đây. Cứ băng cục gạch nào ở lane số 4 mà ko có ở các lane khác là chính nó.

Good luck,

 

[Biologist]

...

7. Heat eppendorf ở 98oC trong 10min. Spin down.

...

bionhien:

Two possibilities: "Membrane-bound proteins" hoac "poor solubility in water"

1) Co phai Ban dang tim cach purify "membrane protein" hay khong? Neu Ban dang lam viec voi "membrane protein" thi E coli khong phai la mot "expression system" tot. Ngoai ra, khi lam viec voi "membrane proteins" thi Ban nen tranh "boil your samples" (as indicated in step 7 above) as this can cause aggregation of proteins.
2) Poor solubility in water-based buffers (e.g. highly hydrophobic proteins): Sau step 7, you should save the pellet in case your recombinant protein is not water-soluble. Co rat nhieu "purification protocols" danh cho "insoluble protein". Ban co the google de tim protocol thich hop cho protein cua ban.

Chuc Ban thanh cong,

 

[Nguyễn Duy Hưng]

Hôm qua bạn có email cho mình nói nó là plasminogen, tiền chất của plasmin, 1 loại serine protease tựa như trypsin.
Mình tra trên Brenda thì MW của nó vào khoảng 80 - 90 kDa, ko biết protein của bạn có thay đổi gì về cấu trúc ko
http://www.brenda-enzymes.org/php/result_flat.php4?ecno=3.4.21.7

 

[nehigoha]

@ bionhien: dark bands là expressed protein hả em?

Để xác định xem mình muốn load bao nhiêu protein/cell lysis trên gel, em cũng có thể thử bằng cách làm pha loãng nhiều cấp độ khác nhau. Không biết mọi người nghĩ sao, chị nghĩ lượng protein em load như hiện tại okie rùi.

Vì vi khuẩn có lớp cell wall nên hiệu suất lyse cell không cao. Nếu em chưa thỏa mãn với cách freeze-thaw rồi heat denature in SDS thì có thể làm thêm vài bước: lyse cell bằng cách sonicate hoặc dùng lysis buffer. Sau khi lyse xong thì spin sample rồi và load supernatant và pellet (tất nhiên là bao gồm cả các bước hoà tan, pha loãng, thêm loading buffer.)

Em lấy ý tưởng express plasminogen bằng bacteria từ đâu thế? Có thể chị biết chưa đủ, nhưng plasminogen là eukaryote excreted protein nên có thể sẽ có modifications. Bacteria chưa chắc có những modifications cần thiết Hơn nữa chaperone của bacteria và eukaryote không giống nhau nên có thể protein sẽ ko fold correctly, và cũng có thể protein bị aggregate trong cell. Vậy nên nếu muốn express plasminogen bằng vk, có lẽ em sẽ phải engineer và thử nhiều gene constructs khác nhau.

Hiện nay, phần lớn plasminogen được tinh chế từ plasma. Chúc em may mắn nhé!

 

[bionhien]

Của em là chất hoạt hóa plasminogen, 72kDa các tham tác em làm giống anh hiếu thế, nhưng trên bản gel không thể nói được gì.

 

[Nguyễn Duy Hưng]

Về bản chất 1 mình gel ko thể nói gì cho em đc. Nó chỉ cho em ước chừng khối lượng của phân tử protein và đánh giá chung về thành phần protein trong mẫu thôi.

Bi giờ em thử ước chừng MW của cái band đậm nhất trong gel của em xem.

Còn em muốn xác định đc có phải protein đó ko thì em vẫn phải có assay thử hoạt tính (enzyme các loại), ELISA hay lai trực tiếp trên gel.

 

[Cao Xuân Hiếu]

bionhien:

Two possibilities: "Membrane-bound proteins" hoac "poor solubility in water"

1) Co phai Ban dang tim cach purify "membrane protein" hay khong? Neu Ban dang lam viec voi "membrane protein" thi E coli khong phai la mot "expression system" tot. Ngoai ra, khi lam viec voi "membrane proteins" thi Ban nen tranh "boil your samples" (as indicated in step 7 above) as this can cause aggregation of proteins.

Quay lại câu chuyện này, kinh nghiệm của tôi

+Đối với protein ở inner membrane thì cách an toàn nhất là heat nhẹ 60oC 10min

+Một số protein bắt buộc phải heat nhẹ vd protein ở Sec machine, nhưng một số inner membrane protein có thể chịu được 95oC 5min

+Protein ở outer membrane thường có cấu trúc b-barrel nên cần heat tối thiểu 95oC 10min hoặc boiling

 

[sinhvienhanoi]

Toi co y kien the này, neu chua ro thi hoi, nhung nguoi dua ra loi khuyen can doc va tim hieu ky, tat viec phat ngon la quyen nhan than cua moi nguoi, nhung de duoc ton trong trong cong dong lam khoa hoc thi thong tin dua ra phai chinh xac,
Quay lai van de bieu hien protein: hien nay hau het cac protein con nguoi ta deu co the express trong E coli voi luong as much as u want, ( co dieu chat luong cac protein co nguon goc mammal bieu hen tren Ecoil thuong khong duoc cao nhu trong human cells vi du nhu cac cyclin dependent protein kinase /CDKs, hoac secret protein gay doc cho ecoli chang han trong truong hop nay chung ta nen chuyen sang dung eukaryotic host)
Truong hop membrane proteins, no la cac hydrophobic protein, nen van de nam o cho lam the nao de hoa tan duoc nhom protein nay (downstream processing) chu khong phai van de o cho bieu hien ra chung (upstream engineering), do vay ban nen chon buffer hop ly, ( vi du buffer co chua aceton nitril chang han, khi can dung trong mot trang thai khac ban co the cho bay hoi eceton nitril de dang ) cai nay toi chua co nhieu experience lam
Con de lua chon mot host express thi hop, can nghien cuu ky phenotype cua host do, cac ban nen vao www.novagen.com (day la cong ty dang so huu T7 expression system)
Vi du su khac biet giua DH5alpha hay BL21 hay BL21 Lys codon plus....

cuc chang da nguoi ta moi chon cac he bieu hien khac (Piachia patosis, insect, CHO) khong phai la ecoli

Quay lai chuyen Plasmidnogen, day la mot mammal protein no rat kho bieu hien tren ecoli, nhung nguoi ta da lam duoc cach day 20 nam roi, co dieu plasminogen duoc encode boi rare codon nen can phai chon duoc host ecoli hop ly, (da duoc incorported with extra rara codons encodes for Arginine, which is in short in EColi) nho do co the de dang express duoc mammal protein,

duoi day la mot vai vi du


The Production of Improved Tissue-Type
Plasminogen Activator in Escherichia coli
Ralf Mattes, Ph.D.1
ABSTRACT
Tissue-type plasminogen activator (t-PA) is a valuable thrombolytic agent because
of its high affinity to fibrin.When produced in mammalian cell lines, it is glycosylated,
a modification that is believed to promote its rapid clearance from the circulation.
Bacteria such as Escherichia coli have been tested as alternative expression systems but
were not able to express the cDNA of t-PA effectively. The coding sequence for t-PA revealed
a significant proportion of AGA and AGG codons, which are rarely used in the
coding sequences of E. coli. The argU and argW gene products of E. coli proved to be
minor tRNAarg species, respectively decoding the very rare triplets AGA/AGG and AGG
for arginine. Analysis of genomic fragments from E. coli for both tRNAarg genes revealed
the presence of defective, cryptic prophages integrated within the impaired tRNA genes.
Cloning and supplementation of the limiting tRNA genes argU and argW on helper plasmids
improved the translation of the rare AGA and AGG codons. This augmentation
improved bacterial growth and enhanced t-PA production in the form of inactive inclusion
bodies. This dependence on augmentation of tRNAarg4 or tRNAarg5 for improved cell
growth and expression was also observed for other genes with a high content of these rare
arginine codons. Construction and production of nonglycosylated t-PA in inclusion bodies
in E. coli along with improvement of the subsequent renaturation and purification procedures
resulted in material comparable to that derived from CHO cells. Deletion of domain-
encoding segments yielded various “muteins” of t-PA (e.g., reteplase [rPA]) that
could be produced in and activated from the purified inclusion bodies analogously. Furthermore,
it was shown that rPA has an extended half-life in the circulation because of its
lack of glycosylation and impaired receptor binding capability. rPA was successfully used
in various clinical studies. It is a new-generation thrombolytic agent with a longer halflife
and can thus be administered more conveniently as a double bolus.
KEYWORDS:Tissue plasminogen activator, Escherichia coli, production, tRNA
augmentation, rPA, t-PA
Objectives: Upon completion of this article, the reader should be able to (1) summarize the differences between traditional tissue-type
plasminogen activator (t-PA) and the genetically engineered product, and (2) recognize the clinical usefulness of the new preparation.
Accreditation: Tufts University School of Medicine is accredited by the Accreditation Council for Continuing Medical Education to
provide continuing medical education for physicians. TUSM takes full responsibility for the content, quality, and scientific integrity of
this continuing education activity.
Credit: Tufts University School of Medicine designates this education activity for a maximum of 1.0 hours credit toward the AMA
Physicians Recognition Award in category one. Each physician should claim only those hours that he/she actually spent in the educational
activity.
Seminars in Thrombosis and Hemostasis, volume 27, number 4, 2001. Address for correspondence and reprint requests: Dr. Ralf Mattes, Institut für
Industrielle Genetik, Universität Stuttgart, Allmandring 31, D-70569 Stuttgart, Germany. E-mail: ralf.mattes@po.uni-stuttgart.de. 1Institut für
Industrielle Genetik, Universität Stuttgart, Stuttgart, Germany. Copyright © 2001 by Thieme Medical Publishers, Inc., 333 Seventh Avenue,
New York, NY 10001, USA.Tel: +1(212) 584-4662. 0094-6176,p;2001,27,04,325,336,ftx,en;sth00733x.


Biosci Biotechnol Biochem. 1999 Dec;63(12):2097-101.

The expression of proUK in Escherichia coli: the vgb promoter replaces IPTG and coexpression of argU compensates for rare codons in a hypoxic induction model.
Jiang L, Yang Y, Chatterjee S, Seidel B, Wolf G, Yang S.

Shanghai Research Center of Biotechnology, Chinese Academy of Sciences, P.R.China. lanjiang@hotmail.com

Abstract
The expression of the proUK gene was improved by the coexpression of the argU gene cloned in a moderate copy number vector. As the proUK gene contains 2% AGG/AGA codons, which is much higher than the normal frequency in E. coli, about 0.14%-0.21%, the argU gene cloned in a multicopy plasmid was coexpressed with the proUK expression vector in our experiments. In E. coli strain BL21(DE3), IPTG is known to induce the expression of T7 RNA polymerase gene and this enzyme can transcribe the proUK gene under the control of the T7 promoter leading to expression of proUK. To replace IPTG by a cheaper alternative on a large scale, we constructed a plasmid in which the vgb promoter--which is known to be activated by the onset of hypoxic conditions--controls the T7RNA polymerase gene expression. Low oxygen conditions were then used to activate the vgb promoter causing T7RNA polymerase gene expression and finally leading to the expression of proUK as inactive inclusion bodies. Our experiments on a large scale in a bioreactor show that the expression of proUK accounts for about 30% of total protein after about 6 h of anaerobic cultivation, so the presented model represents an economical alternative to IPTG induction.



THEJ OURNAOFL B IOLOGICACLH EMISTRY
0 1987 by The American Society of Biological Chemists, Inc
Vol. 262, No. 8, Issue of March 15, pp. 371M725 1987
Printed in d..S.A.
cDNA Cloning and Expression in Escherichia coli of a Plasminogen
Activator Inhibitor from Human Placenta*
(Received for publication, September 8, 1986)
Richard D. YeS6, Tze-Chein Wunll, and J. Evan SadlerSII
From the $Howard Hughes Medical Institute Laboratories and Departments of Medicine and Biological Chemistry, Washington
University School of Medicine, St. Louis, Missouri 63110 and the llMonsanto Company, St. Louis, Missouri 63198
Two nearly full-lengthcD NAs for placentalp lasminogen
activator inhibitor (PAI) have been isolated from
a human placenta Xgtll cDNA library. One positive
(XPAI-75.1) expressed a protein that could adsorb and
purify anti-PA1 antibodies. The expressed protein inhibited
the activity of human urokinase in a fibrin
autography assay, and formead 79-kDa (reduced)c ovalent
complex with 1251-urokinase that could be immunoprecipitated
with anti-PAI. The cDNA insert of
the longer isolate( XPAI-75.15)c onsisted of 1909 base
pairs, including a 5”noncoding region of 55 base pairs,
an open reading frameo f 1245b ase pairs, a stop codon,
a 3’-noncoding region of 581 base pairs, anda poly(A)
tail. The size of the mRNA was estimated to be 2.0
kilobases by Northern blot analysis. The translated
amino acid sequence consisted of 415 amino acids,
corresponding to a 46.6-kDa protein. The sequence
was related to members of the serpin gene family,
particularly ovalbumin and the chicken gene Y protein.
Like these avian proteins, placentaPl A1 appears
to lack a cleavable NHz-terminal signal peptide. Residues
347-376 were identical to the partial sequence
reported recently for a PA1 isolated from the human
monocytic U-937 cell line. Placental PA1 mRNA was
apparently expressed alot w levels in human umbilical
vein endothelial cells, but was not detectableH eipnG 2
hepatoma cells. It was present in U-937ce lls and was
inducible at least 10-fold by phorbol 12-myristate1 3-
acetate. Thus placental PA1is a unique member of the
serpin gene family, distinct from endothelial-PtyApIe.
It is probably identical to monocyte-macrophage PAL


day nua
Journal of Biotechnology, 17 (1991) 109-120
© 1991 Elsevier Science Publishers B.V. (Biomedical Division) 0168-1656/91/$03.50
ADONIS 016816569100052R
109
BIOTEC 00557
High-level secretion of human apolipoprotein E
produced in Escherichia coli: use of a secretion
plasmid containing tandemly polymerized
ompF-hybrid gene
Tatsurou Shibui 1, Michiru Uchida-Kamizono 1, Hiroko Okazaki 2,
Jun Kondo 1, Satoru Murayama 1, Yuuki Morimoto 1, Kenji Nagahari 1
and Yutaka Teranishi 1
1 Biosciences Laboratory and e Toxicology Laboratory, Research Center, Mitsubishi Kasei Corporation,
Kanagawa, Japan
(Received 2 April 1990; revision accepted 3 June 1990)
Summa~
A gene encoding the mature form of human apolipoprotein E (h-apoE) was fused
to the secretion signal coding sequence of the Escherichia coli major outer membrane
protein F (ompF) which was preceded by a consensus Shine-Dalgarno
sequence. Two copies of this hybrid gene were inserted tandemly into an expression
vector and expressed in E. coli under the transcriptional control of two tac
promoters regulated by lac repressors. By the addition of isopropyl-fl-D-thiogalactopyranoside
(IPTG) to the growth media, cells synthesized h-apoE at the level of
27.2 #g per A600 and up to 22% of the total cellular protein. The h-apoE produced
by E. coli was processed precisely, secreted into the periplasmic space and formed
protein aggregates there. However, despite aggregation, they were easily dissolved in
water and actively formed protein-lipid complexes with dimyristdyl phosphatidyl
choline (DMPC). These results demonstrated that E. coli cells are able to synthesize
and secrete a large amount of active h-apoE using a prokaryotic signal sequence.
Escherichia coli; Signal peptide, ompF; Human apoE; Secretion production; Correct

Chuc ban thanh cong

 

[Cao Xuân Hiếu]

Truong hop membrane proteins, no la cac hydrophobic protein, nen van de nam o cho lam the nao de hoa tan duoc nhom protein nay (downstream processing) chu khong phai van de o cho bieu hien ra chung (upstream engineering), do vay ban nen chon buffer hop ly, ( vi du buffer co chua aceton nitril chang han, khi can dung trong mot trang thai khac ban co the cho bay hoi eceton nitril de dang ) cai nay toi chua co nhieu experience lam

Xin cho ví dụ thành phần buffer. Sau khi có protein fraction rồi thì hòa SDS sample buffer ntn? Có heat trước khi điện di SDS-PAGE hay k? Nếu có thì ntn?

 

[sinhvienhanoi]

Ban cao Xuan Hieu co hoi "Xin cho ví dụ thành phần buffer. Sau khi có protein fraction rồi thì hòa SDS sample buffer ntn? Có heat trước khi điện di SDS-PAGE hay k? Nếu có thì ntn? "
Toi xin tra loi rang
Doi voi hydrophobic protein, thi can phai "try and error", u learn it by doing yourself experiments,
Va hinh nhu cai ban hoi khong phai lien quan den van de purify hydrophobic protein ma la chay SDS gel cho no, noi nhu vay thi toi nghi khong co gi dac biet o buoc nay, ma cai kho no nam o cho purify nhom protein nay, nguoi ta se phai thu cac detergent, va nhieu khi ket hop ca mot so dung moi dac biet nua, nhu toi da de cap,ban co the dung aceton nitril (mot dung moi pho biet de chay HPLC) va dung de rua hay hoa tat cac hop chat hydrophobic, con luong cho vao bao nhieu, phan phai tu tim lay, thong thuong co the tu 5 den 60%
ban nen tham khao mot so reference: protein handbooks Humana Press, (toi nghi ban da co trong tay book nay)

hay article duoi day, xin loi ban toi khong biet lam the nao de attach duoc PDF vao post nay, nen neu ban can toi se co the email
chuc ban thanh cong

International Journal of Biological Macromolecules 39 (2006) 83–87
A simple strategy towards membrane protein purification
and crystallization

Damian Niegowski a,b, Marie Hedr´en a, P¨ar Nordlund a, Said Eshaghi a,∗
a Department of Medical Biochemistry and Biophysics, Karolinska Institutet, SE-171 77 Stockholm, Sweden
b Department of Biochemistry and Biophysics, Arrhenius Laboratories for Natural Sciences, Stockholm University, SE-106 91 Stockholm, Sweden
Received 11 November 2005; received in revised form 13 December 2005; accepted 9 February 2006
Available online 23 February 2006
Abstract
A simple and cost-efficient detergent screening strategy has been developed, by which a number of detergents were screened for their efficiency
to extract and purify the recombinant ammonium/ammonia channel, AmtB, from Escherichia coli, hence selecting the most efficient detergents
prior to large-scale protein production and crystallization. The method requires 1ml cell culture and is a combination of immobilized metal ion
affinity chromatography and filtration steps in 96-well plates. Large-scale protein purification and subsequent crystallization screening resulted
in AmtB crystals diffracting to low resolution with three detergents. This strategy allows exclusion of detergents with the lowest probability in
yielding protein crystals and selecting those with higher probability, hence, reducing the number of detergents to be screened prior to large-scale
membrane protein purification and perhaps also crystallization.
© 2006 Elsevier B.V. All rights reserved.
Keywords: Membrane proteins; Detergent screen; High-throughput
1. Introduction
The recombinant expression and subsequent purification of
integral membrane proteins are considered major challenges,
and together with the crystallization step, the major hurdles
towards routine structure determination of membrane proteins.
Consequently, the number of membrane proteins with known
structure has remained negligible as compared to those of soluble
proteins [1,2]. This in turn causes serious lack of information
in the field of drug discovery, since membrane proteins already
cover more than 50% of the current drug targets [3,4]. Therefore,
it is essential to improve the success rate in membrane
proteins structural determination, by dealing with experimental
difficulties in the production of these proteins.
Experimental procedures for handling and isolating integral
membrane proteins are generally more challenging than their
soluble counterparts, since the former requires purification in
detergent. General experiences from workers in the field with

This paper was presented at the “Challenging Proteins Workshop” in Paris,
October 17–18, 2005.
∗ Corresponding author. Tel.: +46 8 524 86863; fax: +46 8 524 868650.
E-mail address: said.eshaghi@ki.se (S. Eshaghi).
the problematic experimental behaviour of integral membrane
proteins have lead to the expectation that these proteins are dramatically
harder to produce than soluble proteins. One of the
reasons may be the usage of the wrong detergent during extraction
and purification. There are dozens of different detergents
that are commonly used, dozens more that are less characterized
but still probably useful, and many novel detergents under
development. It has also been reported that some compartments
of the cell membrane show resistance towards certain detergents
[5]. Moreover, mixtures of detergents are sometimes used during
purification and crystallization [6,7]. Altogether, the size
of the detergent parameter space becomes very large. Therefore,
it is crucial to choose the right detergent for an efficient
extraction and purification of the membrane protein of interest.
Recently, we reported an efficient strategy, by which we could
screen the expression of a number of membrane proteins in a
high-throughput manner [8]. Here, we report the application of
this strategy to design downstream protocols for large-scale production
of the recombinantly expressed ammonium transporter
AmtB from Escherichia coli, by which 26 detergents, 4 types
of chromatography columns and various buffer conditions have
been screened using a 96-well plate format. The method is very
cost efficient and may easily be applied to other membrane pro-
0141-8130/$ – see front matter © 2006 Elsevier B.V. All rights reserved.
doi:10.1016/j.ijbiomac.2006.02.011
84 D. Niegowski et al. / International Journal of Biological Macromolecules 39 (2006) 83–87
teins. In addition, we have tested the feasibility of using this platform
for choosing the right detergent for crystallization attempts.
We believe that using the presented strategy will minimize the
number of detergent candidates in initial crystallization screens,
by excluding those that will yield low amount of proteins.
2. Materials and methods
2.1. Materials
All the detergents were purchased from Anatrace (OH, USA).
2.2. Methods
2.2.1. Cloning
Coding sequences for the AmtB was obtained from SwissProt
database and used for primer design usingSGDWebprimer
design program. The cloning was performed as described in
[8]. Briefly, touchdown PCR was performed using Platinum
PfxDNApolymerase (Invitrogen, Stockholm, Sweden); primers
containing at least 15 gene-specific nucleotides (TAG Copenhagen,
http://www.tagc.com); and the E. coli template K12

isolated with High Pure PCR Template Preparation Kit (Roche,
Stockholm, Sweden).
Another PCRwas performed using the same Pfx polymerase,
primers containing attB sites (Invitrogen), and the PCR products
from the touchdown reactions as templates. The linear fragments
flanked by attB-sequences were subjected to site-specific recombination
with pDONR201 vector (Invitrogen), containing the
ccdB gene, flanked by attP sites and catalyzed by BP Clonase
(see manufacturer’s protocols) yielding entry clones. The entry
clones were subjected to another round of site-specific recombination
catalyzed by the LR Clonase enzyme mix (Invitrogen) in
order to subclone the genes of interest into the destination vector
(AstraZeneca, S¨odert¨alje, Sweden) containing the ccdB gene
flanked by attR sites, as well as the coding sequences for fusion
tags N-terminal FLAG and C-terminal 6-His (see Invitrogen’s
protocols).
The resulting expression constructs were used to transform
E. coli C41(DE3) (Avidis, Saint-Beauzire, France). Construct
identity was verified by dideoxysequencing.
2.2.2. Protein overexpression and detergent screening
The cells were grown in a shake flask at 37 ◦C until the cultures
reached the OD600 of ∼0.8. The culture was then cooled
down to 20 ◦C and induced overnight with 0.1mMisopropyl--
d-1-thiogalactoside. Aliquots of 1ml were added to a 96-well
plate and harvested by centrifugation at 3000×g for 10 min.
The overall procedure is outlined in Fig. 1. The cell pellets
were resuspended in 50 l 20mM Tris–HCl pH 8.0, 50mM
NaCl, 0.5mM Tris(2-carboxyethyl)phosphine hydrochloride
(TCEP), 1 mg/ml lysozyme, complete protease inhibitor cocktail
EDTA-free (Roche), 10 units/ml benzonase (VWR International),
and the appropriate detergent at concentrations 1–2%
according to Table 1, respectively. Lysis and extraction were
performed for 1 h at 4 ◦C. The suspensionwas filtered using a 96-
well filter plate (Millipore, Stockholm, Sweden). The filtratewas
Fig. 1. An overall scheme of the detergent screen platform using 96-well plates.
added to 25l Ni-NTA agarose resin (Qiagen, Stockholm, Sweden)
pre-equilibrated with purification buffer (P-buffer) containing
20mMTris–HCl pH 8.0, 300mMNaCl, 0.5mMTCEP, and
the appropriate detergent. After 15 min agitation at 4 ◦C, the
unbound materialwas removed by 30 s centrifugation at 100×g.
The resinwas thenwashed with 20 column volumes (CV) 40mM
imidazole in the P-buffer containing the appropriate detergent
at 100×g for 30 s. The bound recombinant membrane proteins
Table 1
Detergents and their concentrations used in the screen
Detergent name Abbreviation CMC (mM) Extraction (mM)
FOS-CHOLINE-10 FC10 11 63 (2)
FOS-CHOLINE-11 FC11 1.85 30 (1)
FOS-CHOLINE-12 FC12 1.5 32 (1)
HEGA-10 HEGA-10 7 54 (2)
Nonyl maltoside NM 6 43 (2)
Decyl maltoside DM 1.8 21 (1)
Undecyl maltoside UDM 0.59 20 (1)
Dodecyl maltoside DDM 0.17 20 (1)
CHAPS CHAPS 8 32 (2)
CHAPSO CHAPSO 8 32 (2)
Nonyl thiomaltoside NTM 3.2 32 (1.5)
Decyl thiomaltoside DTM 0.9 20 (1)
Undecyl thiomaltoside UDTM 0.21 19 (1)
Dodecyl thiomaltoside DDTM 0.05 1.9 (1)
Cymal-6 Cy6 0.56 20 (1)
Cymal-7 Cy7 0.19 19 (1)
LDAO LDAO 1 43 (1)
TDAO TDAO 0.29 39 (1)
C8E4 C8E4 8 64 (2)
C8E6 C8E6 10 51 (2)
C10E5 C10E5 0.81 26 (1)
C12E8 C12E8 0.09 19 (1)
Octyl glucoside OG 18 68 (2)
Nonyl glucoside NG 6.5 65 (2)
Triton X-100 TX100 0.23 15 (1)
Triton X-114 TX114 0.20 36 (2)
Values in parenthesis indicate percentages.
D. Niegowski et al. / International Journal of Biological Macromolecules 39 (2006) 83–87 85
were finally recovered in 30 l P-buffer containing 500mMimidazole
and the respective detergent, by centrifugation at 100×g
for 1 min. The eluted material was then analyzed by dot blot.
2.2.3. Large-scale protein purification
Cultures were grown in baffled shake flasks as described
above, and finally harvested by centrifugation at 7000×g for
15 min. Cell pellets were resuspended in 20mM Tris–HCl
pH 8.0, 50mM NaCl, 0.5mM TCEP, 10 u/ml benzonase and
1 mg/ml lysozyme, sonicated and centrifuged at 15,000×g for
10 min to remove cell debris. Cell membranes were finally harvested
by 1 h centrifugation at 150,000×g. The membranes
were resuspended and solubilized with 1% FC12 detergent
in the P-buffer supplemented with 20mM imidazole using a
glass homogenizer, followed by centrifugation for 45 min at
200,000×g to remove unsolubilized material. The clear supernatants
containing solubilized membrane proteins were loaded
on TALON resin pre-equilibrated with the P-buffer, including
20mM imidazole and 0.1% FC12. The resin was washed once
with 15 CV P-buffer containing 20mM imidazole and 0.1%
FC12. When detergent exchanged was desired, 5 CV wash with
0.1% FC12 was performed followed by 10 CV wash with the
appropriate detergent. The recombinant proteins were eluted
with 250mM imidazole in the wash buffer. The IMAC purified
AmtBwas further polished by gel filtration using a Superdex 200
column (GE-Healthcare, Uppsala, Sweden) in 20mMTris–HCl
pH 8.0, 150mMNaCl, 0.5mMTCEP and the appropriate detergent.
2.2.4. Dot blot and SDS-PAGE
One microlitre of sample was applied to nitrocellulose and
allowed to dry. The 6-His-tagged proteins were detected using
INDIA HisProbe-HRP Western blotting probe (Pierce, Stockholm,
Sweden) according to the manufacturer’s protocol. The
signals were detected with FluorS-multiImager (BioRad, Stockholm,
Sweden) and quantified using the Quantity One software
(BioRad). The purity of the expressed proteins was monitored
by SDS–PAGE, using Nu-PAGE 4–12% Bis–Tris-gels (Invitrogen).
2.2.5. Crystallization
The purified proteins were concentrated using Amicon Ultra
100-kDa cut-off (Millipore) to a protein concentration of
4–5 mg/ml. Crystallization was performed by sitting-drop vapor
diffusion at 20 ◦C at a ratio of 1:1. Protein crystals were grown
with undecyl maltoside (0.1%), dodecyl maltoside (0.03%) or
Cymal-6 (0.06%), in either 12% PEG 4000 or 30% PEG 400
buffered with 100mM MOPS pH 7.0 (MbClass II screen, Nextal
Biotechnologies, Montreal, Canada).
3. Results
Prior to large-scale purification and subsequent crystallization,
we applied the previously reported detergent screening
strategy [8] in order to explore and refine the extraction and
purification of AmtB. Recombinant AmtB was overexpressed
in a shake flask to ensure equality of the starting material prior
Fig. 2. Detergent screen analysis histograms of AmtB. From left to right: (1)
FC10, (2) FC11, (3) FC12, (4) HEGA10, (5) NM, (6) DM, (7) UDM, (8) DDM,
(9) CHAPS, (10) CHAPSO, (11) NTM, (12) DTM, (13) UDTM, (14) DDTM,
(15) LDAO, (16) TDAO, (17) C8E4, (18) C8E6, (19) C10E5, (20) C12E8, (21)
OG, (22) NG, (23) TX100, (24) TX114.
to further processing with various detergents. Twenty six detergents,
each at final concentrations of 1–2% were screened, to
find the best detergent and detergent concentration required for
an efficient protein extraction. These detergents either belong to
families whose members have been successfully used to produce
crystals, such as maltosides and glucosides [9], or are commonly
used for protein purification in many laboratories, such as Triton
and CHAPS, in addition to some rather new and uncharacterized,
such as cymals. Using a 96-well plate, cell cultures in 1ml
aliquots were lysed and solubilized simultaneously. Solubilized
membrane proteins and the soluble content of the cells were
successfully separated from cell debris and inclusion bodies by
filtration, as previously described [8,10]. Using the small-scale
His-tag affinity purification, we were able to discard any AmtB
that was partially solubilized, i.e. containing membrane fragments
due to incomplete solubilization, or precipitated, and thus,
the yield of actual native and solubilized protein could be estimated
by dot blot analysis (Fig. 2). Interestingly, the yield of
purified AmtB changed with different detergents. In addition,
for some detergents, an increase in the concentration resulted
in more purified protein, whereas with other detergents such
increase would reduce the yield (data not shown). The latter
would suggest the destabilization effect of certain detergents on
specific membrane proteins, due to, e.g. excessive delipidation
[11–13].
The same platform was used to perform purification optimizations.
To this end, we investigated the various imidazole
concentrations during purification steps in combination with
four different types of metal affinity columns, to find the optimum
purification conditions prior to large-scale purifications
(Fig. 3). The dot blot analysis of the multi-parameter screen
indicated that presence of imidazole during binding improves
the yield of AmtB. Moreover, the TALONresin seemed to purify
AmtB more efficiently than others. Although a second elution
step showed the presence of more material in other columns
than TALON, we decided to use TALON resin for our largescale
purifications, since SDS-PAGE analysis of eluted material
showed purer material coming off TALON (data not shown).
The same procedures as small-scale protein purification were
used to produce milligrams of pure AmtB, suitable for crystallization
trials. However, ultracentrifugation steps were intro86
D. Niegowski et al. / International Journal of Biological Macromolecules 39 (2006) 83–87
Fig. 3. AmtB purification optimization. AmtB was extracted with FC12 (F),
DDM (D) and TX100 (T). Imidazole was used during binding at concentrations
0mM (1 and 2) and 20mM (3 and 4), and during washing at concentrations
20mM(1 and 3) and 40mM(2 and 4). Column volumes used were 25 and 50 l
Ni-NTA agarose in A and B, respectively, following in the same way by Ni-NTA
superflow (Qiagen) (C and D), Ni-sepharose fast flow (GE-Healthcare) (E and
F) and TALON (Clontech, Stockholm Sweden) (G and H), respectively.
duced to increase the purity and maintain the high protein yield.
One percent FC12 was used to initiate the purification, as this
detergent gave the highest purification yield of AmtB. Detergent
exchange was successfully performed during IMAC purifica-
Fig. 4. Gel filtration (A) and SDS-PAGE analysis (B) of AmtB after extraction
with FC12 and further purification with DDM. The peak marked with asterisk
was submitted to SDS-PAGE showing presence of pure AmtB. The other peaks
contained either impurities or no protein.
Fig. 5. AmtB crystals grown in the presence of DDM (A) and Cymal-6 (B).
tion followed by gel filtration to further purify AmtB to higher
homogeneity, and finally the purity of the sample was verified
by SDS-PAGE (Fig. 4). Although, some of the detergents, as
indicated in Fig. 2, showed low efficiency in extracting AmtB,
we decided to include these detergents in the large-scale production
processes to further explore their effects during purification
and subsequent crystallization. Thus, AmtB was extracted with
FC12 and subsequently purified with FC12, UDM, DDM, Cy6,
Cy7, OG and LDAO. AmtB crystals appeared in the first screen
after three days in the presence of DDM and Cymal-6 (Fig. 5).
The crystals could diffract poorly to ∼11A° .
AmtB could not be crystallized in the presence of other detergents,
except for UDM in which micro-crystals were grown.
4. Discussion
To produce high quantities of pure native membrane proteins
has always been a major obstacle in crystal structure determination
of membrane proteins. This problem has so far been
connected to lowexpression of recombinant membrane proteins.
However, we have shown here that this problem may also be due
to poor understanding of purification procedures, namely the
usage of wrong detergents. If commonly used detergents such
as Triton X-100, octyl glucoside or CHAPS would have been
D. Niegowski et al. / International Journal of Biological Macromolecules 39 (2006) 83–87 87
used in the present study, the results would be no or very poor
yields of recombinantly produced AmtB, and a poor expression
was wrongly assumed. In addition, screening of many detergents
during crystallization has been shown to be highly important for
obtaining high-quality crystals necessary for solving the structure
of membrane proteins [7,14].
Due to the rather high cost of detergents, traditional methods
for screening various detergents and purification optimizations,
i.e. membrane preparation by ultracentrifugation and further
protein purification and analysis by gel filtration, SDS-PAGE
and Western blotting, is both expensive and time consuming.
We believe the use of present screening procedure, allowing
tens of various purification strategies and detergent screening
at microlitre volumes, and subsequent analysis by dot blot, will
minimize the costs, thus, enabling more thorough optimizations
prior to tedious large-scale membrane protein production. It is
important to remember that the small-scale purification platform
has an elevated degree of initial impurities due to the presence of
soluble as well as membrane proteins, as compared with purification
following membrane isolation. Therefore, any progress
with purification during this step may provide important information,
such as required detergent concentration or critical salt
concentration, for large-scale preparative steps, and thus be of
great advantage.
There is an interesting correlation between the yield of
extracted protein using a certain detergent and its ability to crystallize
in that detergent: UDM, DDM and Cy6 were efficient
in protein extraction and they facilitated crystal growth, while
neither OG nor LDAO could extract sufficient protein and no
crystals were grown in their presence. To suggest that detergents
highly efficient in extracting a certain protein would facilitate
crystallization of that protein is currently rather impossible and
many more studies are required to validate that. However, to
exclude detergents that are not useful for high-yield extraction
of a specific protein (e.g. due to destabilizing the protein) may be
very helpful to minimize the number of detergents during crystallization
screening. The fact that no crystals of AmtB were
grown in the presence of OG and LDAO may be such an indication.
The structure of AmtB was recently solved to high resolution
[15,16]. In those studies, AmtB crystals were grown in the presence
of OG and LDAO, respectively. Interestingly, none of these
detergents could help to produce AmtB crystals in our study.
Khademi et al. reported the extraction of AmtB with almost
10% OG (200 mM), with subsequent purification using 1% of
the same detergent. Our attempt to perform the same procedure
for isolating AmtB did not result in any crystals. Since it
is rather unclear exactly how Khademi et al. purified and crystallized
AmtB, the comparison of the procedures are difficult.
There is also no information from these reports whether the used
detergents in the crystallization were also the best detergents in
extracting AmtB. The differences between the constructs used
in all three studies may be the reason for the differences in crystallization
behaviour of AmtB, as our construct contains a FLAG
followed by an attB-site and a TEV-protease cleavage site at the
N-terminus, which, together with the nature of the used detergent,
may play important role for crystal contacts. The other
two constructs lack this long N-terminal tag. Khademi et al.
have crystallized a protein lacking the first transmembrane helix
and containing two mutations.
We have successfully applied this strategy to 10 other membrane
proteins, out of two have so far resulted in diffracting
crystals.
We believe the presented platform is indeed an efficient tool
for benchmarking and optimizing important purification parameters,
e.g. the type and concentration of detergents, buffer composition
and column material, in a membrane protein production
and crystallization pipe-line. The choice of the right detergent
is indeed one of the important keys for membrane protein stability
and crystallization. However, due to the large number of
detergents available in the market, it is an elaborate and expensive
task to choose the right detergent(s) for purification and
crystallization of the target protein, by traditional methods, if
one determines to screen a large number of detergents. On the
other hand, screening fewer detergents may result in poor yield,
unstable protein and/or no protein crystals, and is not recommended.
Thus, the presented strategy allows the screening of
tens of detergents, for their efficiency of pure protein production
and crystallization, easily and simultaneously, producing
reliable and reproducible results, at very low cost.
Acknowledgement
The European Membrane Protein Consortium (E-MEP), the
Swedish Research Council and theG¨oran Gustafsson foundation
are acknowledged for financial support.
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Hoac

 

[Cao Xuân Hiếu]

Ban cao Xuan Hieu co hoi "Xin cho ví dụ thành phần buffer. Sau khi có protein fraction rồi thì hòa SDS sample buffer ntn? Có heat trước khi điện di SDS-PAGE hay k? Nếu có thì ntn? "
Toi xin tra loi rang
Doi voi hydrophobic protein, thi can phai "try and error", u learn it by doing yourself experiments,
Va hinh nhu cai ban hoi khong phai lien quan den van de purify hydrophobic protein ma la chay SDS gel cho no, noi nhu vay thi toi nghi khong co gi dac biet o buoc nay, ma cai kho no nam o cho purify nhom protein nay, nguoi ta se phai thu cac detergent, va nhieu khi ket hop ca mot so dung moi dac biet nua, nhu toi da de cap,ban co the dung aceton nitril (mot dung moi pho biet de chay HPLC) va dung de rua hay hoa tat cac hop chat hydrophobic, con luong cho vao bao nhieu, phan phai tu tim lay, thong thuong co the tu 5 den 60%

cùng là dân làm MS sao lại ko biết aceton nitril. Vấn đề của ng khởi đầu topic này là họ biểu hiện gene trong E.coli nhưng khi load sample lên bản SDS-PAGE thì ko nhìn thấy band biểu hiện. Thế rồi câu chuyện rẽ sang 1 nhánh là nếu protein of interest mà là protein màng thì phải làm sao (heat thế nào để ko bị đóng vón) để điện di SDS-PAGE nhìn thấy band. Giờ bạn muốn tiếp tục rẽ sang hướng tách chiết thì có lẽ nên mở topic riêng vì quá xa câu hỏi ban đầu.