| 出品公司: | ZYbscience |
|---|---|
| 载体名称: | pBacPAK8 |
| 质粒类型: | 昆虫表达载体;杆状病毒表达载体 |
| 克隆方法: | 限制酶,多克隆位点 |
| 启动子: | Polyhedrin |
| 载体大小: | 5538 bp |
| 5' 测序引物及序列: | Bac1 Primer: AACCATCTCGCAAATAAATA |
| 3' 测序引物及序列: | Bac2 Primer: ACGCACAGAATCTAGCGCTT |
| 载体标签: | 无标签 |
| 载体抗性: | 氨苄青霉素 |
| 真核筛选标记: | 无 |
| 克隆菌株: | TOP10 |
| 宿主细胞(系): | 果蝇细胞系 IPLB-Sf21 |
| 备注: | 相关载体 pBacPAK8-His |
| 产品目录号: | ZY631402 |
| 瞬表达/稳表达: | 稳表达 |
| 组成型/诱导型: | 组成型 |
| 病毒/非病毒: | 杆状病毒 |
- ¥3500
- ZYbscience
- 中国/美国
- ZY631402
- 2025年07月07日
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- 详细信息
- 文献和实验
- 技术资料
- 保存条件:
-20℃低温保存
- 保质期:
三年
- 英文名:
pBacPAK8
- 库存:
20
- 供应商:
泽叶生物
载体基本信息
载体质粒图谱和多克隆位点信息
载体简介
载体描述: Available as part of the BacPAK Baculovirus Expression System (Cat. No. 631402). pBacPAK8 is a transfer vector designed for high-level expression of a cloned gene driven by the strong AcMNPV polyhedrin promoter. Flanking AcMNPV sequences allow recombination with viral DNA to transfer the expression cassette to the polyhedrin locus of the viral DNA. The polyhedrin coding sequences have been replaced by a multiple cloning site with 18 unique sites that facilitate the insertion of foreign genes in the correct orientation for expression. The Pac I site at the end of the MCS region provides translational stop codons in all three reading frames for expression of truncated proteins. pBacPAK8 has a pUC origin of replication, an M13 origin for single-stranded DNA production, and an ampicillin resistance gene for selection in E. coli. 1 杆状病毒表达系统简介 Baculovirus gene expression is a popular method for producing large quantities of recombinant proteins in insect host cells. In most cases, posttranslational processing of eukaryotic proteins expressed in insect cells is similar to protein processing in mammalian cells. As a result, insect cell-processed proteins have comparable biological activities and immunological reactivities to proteins expressed in mammalian cells. Protein yields from baculovirus systems are higher, and costs are significantly lower than in mammalian expression systems. The baculovirus expression system can express genes from bacteria, viruses, plants, and mammals at levels from 1–500 mg/liter; most proteins are expressed in the 10–100 mg/liter range, although making predictions is difficult. The baculovirus most commonly used to express foreign proteins is Autographa californica nuclear polyhedrosis virus (AcMNPV). AcMNPV can be propagated in certain insect cell lines; the virus enters the cells and replication begins approximately 6 hours post-infection (h.p.i.). At approximately 20–48 h.p.i., transcription of nearly all genes ceases. The viral polyhedrin and p10 genes, however, are transcribed at high rates. The polyhedrin protein is essential for propagation of the virus in its natural habitat; however, in cell culture, polyhedrin is not needed, and its coding sequence can be replaced with a sequence for a target protein. Hence, the powerful polyhedrin promoter can drive high-level transcription of the insert, resulting in expression of a recombinant protein that can account for over 30% of total cellular protein. The large 134 kb-size of the AcMNPV genome, makes direct manipulation of it difficult, so recombinant baculovirus expression vectors are constructed in two steps (Figure 1). First, a target gene is cloned into a modified polyhedrin locus contained in a relatively small transfer vector (<10 kb). The polyhedrin coding sequence has been deleted and replaced with a multiple cloning site (MCS). A target gene is inserted into this MCS, between the polyhedrin promoter and polyadenylation signals. Transfer vectors also contain a plasmid origin of replication and an antibiotic resistance gene for propagation in E. coli, but they are unable to replicate in insect cells. In the second step, the transfer vector and a viral expression vector are cotransfected into insect cells. Double recombination between viral sequences in the transfer vector and the corresponding sequences in the viral DNA transfers the target gene to the viral genome. The BacPAK Baculovirus Expression System uses BacPAK6, a specially engineered virus that facilitates construction and selection of recombinant expression vectors. BacPAK6 has an essential gene adjacent to the polyhedrin locus that provides selection for recombinant viruses. Sites for Bsu36 I, which does not cut wild-type AcMNPV DNA, were introduced into the genes flanking the polyhedrin expression locus of BacPAK6. Digesting BacPAK6 with Bsu36 I releases two fragments. The first carries part of a downstream gene, ORF1629, that is essential for viral replication. If the second large DNA fragment recircularizes by itself, the resulting viral DNA will lack an essential part of the genome and be unable to produce viable viruses. However, the transfer vector carries the missing ORF1629 sequence, and if the large fragment recombines with it, the resulting circular DNA will contain all the genes necessary for viral replication. This double recombination event restores the essential gene and transfers the target gene from the transfer vector to the viral genome. Cotransfections using Bsu36 I-digested BacPAK6 viral DNA produce recombinant viruses at frequencies approaching 100%. This User Manual contains directions for establishing insect cell cultures, as well as for isolating a recombinant baculovirus expression vector using the BacPAK system. More extensive protocols for using baculovirus expression systems are in the baculovirus laboratory manuals 2.实验流程 Obtain insect cell media and establish Sf21 cell line. This step will take3–4 weeks. Maintain working stocks of Sf21 cells. When the stock of cells has been passaged twice, freeze aliquots for long-term storage in liquid nitrogen. Aliquots of frozen cells provide a back-up in case the working stock dies or becomes contaminated. Frozen cells are also a source of fresh cells for replacing working stocks as they become old. Isolating pure recombinant virus requires good viral plaques. Therefore, developing a good plaque assay technique before working with recombinant viruses is advisable.Practice assaying viral plaques. Insert target gene into transfer vector and prepare plasmid DNA. Produce a recombinant virus by cotransfecting Sf21 cells with BacPAK6 viral DNA and the transfer vector-target gene clone. Perform plaque assays on the cotransfection supernatant to obtain individual viral plaques. Test the putative recombinant viruses to confirm that they have incorporated the target gene and/or express the target protein. Amplify recombinant viruses to obtain working stocks. Titer amplified virus stock. Perform small-scale infections to characterize gene expression and to determine the optimum harvest time and infection ratio that will give maximum protein yield. Scale-up: produce target protein in large quantities by infecting larger batches of insect cells.
载体序列
NOTE: The attached sequence file has been compiled from information in the sequence databases,published literature, and other sources, together with partial sequences obtained by Clontech. This vector has not been completely sequenced.
LOCUS pBacPAK8 5538 bp DNA SYN
DEFINITION pBacPAK8
ACCESSION
KEYWORDS
SOURCE
ORGANISM other sequences; artificial sequences; vectors.
FEATURES Location/Qualifiers
source 1..5538
/organism="pBacPAK8"
/mol_type="other DNA"
misc_feature 1..1147
/label="Ac_5_flank"
CDS complement(489..1094)
/label="ORF frame 2"
promoter 1148..1248
/label="PH_promoter"
misc_feature 1174..1191
/label="polyhedrin_fwd_primer"
misc_feature 1337..2770
/label="Ac_3_flank"
CDS complement(1353..2606)
/label="ORF frame 2"
misc_feature complement(1435..2233)
/label="r_ORF1629"
rep_origin 2858..3164
/label="f1_origin"
misc_feature 3432..3454
/label="pGEX_3_primer"
promoter 3613..3641
/label="AmpR_promoter"
gene 3683..4543
/label="Ampicillin"
/gene="Ampicillin"
CDS 3683..4543
/label="ORF frame 2"
rep_origin 4698..5317
/label="pBR322_origin"
ORIGIN
1 aacggctccg cccactatta atgaaattaa aaattccaat tttaaaaaac gcagcaagag
61 aaacatttgt atgaaagaat gcgtagaagg aaagaaaaat gtcgtcgaca tgctgaacaa
121 caagattaat atgcctccgt gtataaaaaa aatattgaac gatttgaaag aaaacaatgt
181 accgcgcggc ggtatgtaca ggaagaggtt tatactaaac tgttacattg caaacgtggt
241 ttcgtgtgcc aagtgtgaaa accgatgttt aatcaaggct ctgacgcatt tctacaacca
301 cgactccaag tgtgtgggtg aagtcatgca tcttttaatc aaatcccaag atgtgtataa
361 accaccaaac tgccaaaaaa tgaaaactgt cgacaagctc tgtccgtttg ctggcaactg
421 caagggtctc aatcctattt gtaattattg aataataaaa caattataaa tgctaaattt
481 gttttttatt aacgatacaa accaaacgca acaagaacat ttgtagtatt atctataatt
541 gaaaacgcgt agttataatc gctgaggtaa tatttaaaat cattttcaaa tgattcacag
601 ttaatttgcg acaatataat tttattttca cataaactag acgccttgtc gtcttcttct
661 tcgtattcct tctctttttc atttttctcc tcataaaaat taacatagtt attatcgtat
721 ccatatatgt atctatcgta tagagtaaat tttttgttgt cataaatata tatgtctttt
781 ttaatggggt gtatagtacc gctgcgcata gtttttctgt aatttacaac agtgctattt
841 tctggtagtt cttcggagtg tgttgcttta attattaaat ttatataatc aatgaatttg
901 ggatcgtcgg ttttgtacaa tatgttgccg gcatagtacg cagcttcttc tagttcaatt
961 acaccatttt ttagcagcac cggattaaca taactttcca aaatgttgta cgaaccgtta
1021 aacaaaaaca gttcacctcc cttttctata ctattgtctg cgagcagttg tttgttgtta
1081 aaaataacag ccattgtaat gagacgcaca aactaatatc acaaactgga aatgtctatc
1141 aatatatagt tgctgatatc atggagataa ttaaaatgat aaccatctcg caaataaata
1201 agtattttac tgttttcgta acagttttgt aataaaaaaa cctataaata cggatccctg
1261 caggcctcga gttcgaatct agaagatctg gtaccgagct cgaattcccg ggcggccgct
1321 taattaattg atccgggtta ttagtacatt tattaagcgc tagattctgt gcgttgttga
1381 tttacagaca attgttgtac gtattttaat aattcattaa atttataatc tttagggtgg
1441 tatgttagag cgaaaatcaa atgattttca gcgtctttat atctgaattt aaatattaaa
1501 tcctcaatag atttgtaaaa taggtttcga ttagtttcaa acaagggttg tttttccgaa
1561 ccgatggctg gactatctaa tggattttcg ctcaacgcca caaaacttgc caaatcttgt
1621 agcagcaatc tagctttgtc gatattcgtt tgtgttttgt tttgtaataa aggttcgacg
1681 tcgttcaaaa tattatgcgc ttttgtattt ctttcatcac tgtcgttagt gtacaattga
1741 ctcgacgtaa acacgttaaa taaagcttgg acatatttaa catcgggcgt gttagcttta
1801 ttaggccgat tatcgtcgtc gtcccaaccc tcgtcgttag aagttgcttc cgaagacgat
1861 tttgccatag ccacacgacg cctattaatt gtgtcggcta acacgtccgc gatcaaattt
1921 gtagttgagc tttttggaat tatttctgat tgcgggcgtt tttgggcggg tttcaatcta
1981 actgtgcccg attttaattc agacaacacg ttagaaagcg atggtgcagg cggtggtaac
2041 atttcagacg gcaaatctac taatggcggc ggtggtggag ctgatgataa atctaccatc
2101 ggtggaggcg caggcggggc tggcggcgga ggcggaggcg gaggtggtgg cggtgatgca
2161 gacggcggtt taggctcaaa tgtctcttta ggcaacacag tcggcacctc aactattgta
2221 ctggtttcgg gcgccgtttt tggtttgacc ggtctgagac gagtgcgatt tttttcgttt
2281 ctaatagctt ccaacaattg ttgtctgtcg tctaaaggtg cagcgggttg aggttccgtc
2341 ggcattggtg gagcgggcgg caattcagac atcgatggtg gtggtggtgg tggaggcgct
2401 ggaatgttag gcacgggaga aggtggtggc ggcggtgccg ccggtataat ttgttctggt
2461 ttagtttgtt cgcgcacgat tgtgggcacc ggcgcaggcg ccgctggctg cacaacggaa
2521 ggtcgtctgc ttcgaggcag cgcttggggt ggtggcaatt caatattata attggaatac
2581 aaatcgtaaa aatctgctat aagcattgta atttcgctat cgtttaccgt gccgatattt
2641 aacaaccgct caatgtaagc aattgtattg taaagagatt gtctcaagct cggatcgatc
2701 ccgcacgccg ataacaagcc ttttcatttt tactacagca ttgtagtggc gagacacttc
2761 gctgtcgtcg cctgatgcgg tattttctcc ttacgcatct gtgcggtatt tcacaccgca
2821 tacgtcaaag caaccatagt acgcgccctg tagcggcgca ttaagcgcgg cgggtgtggt
2881 ggttacgcgc agcgtgaccg ctacacttgc cagcgcccta gcgcccgctc ctttcgcttt
2941 cttcccttcc tttctcgcca cgttcgccgg ctttccccgt caagctctaa atcgggggct
3001 ccctttaggg ttccgattta gtgctttacg gcacctcgac cccaaaaaac ttgatttggg
3061 tgatggttca cgtagtgggc catcgccctg atagacggtt tttcgccctt tgacgttgga
3121 gtccacgttc tttaatagtg gactcttgtt ccaaactgga acaacactca accctatctc
3181 gggctattct tttgatttat aagggatttt gccgatttcg gcctattggt taaaaaatga
3241 gctgatttaa caaaaattta acgcgaattt taacaaaata ttaacgttta caattttatg
3301 gtgcactctc agtacaatct gctctgatgc cgcatagtta agccagcccc gacacccgcc
3361 aacacccgct gacgcgccct gacgggcttg tctgctcccg gcatccgctt acagacaagc
3421 tgtgaccgtc tccgggagct gcatgtgtca gaggttttca ccgtcatcac cgaaacgcgc
3481 gagacgaaag ggcctcgtga tacgcctatt tttataggtt aatgtcatga taataatggt
3541 ttcttagacg tcaggtggca cttttcgggg aaatgtgcgc ggaaccccta tttgtttatt
3601 tttctaaata cattcaaata tgtatccgct catgagacaa taaccctgat aaatgcttca
3661 ataatattga aaaaggaaga gtatgagtat tcaacatttc cgtgtcgccc ttattccctt
3721 ttttgcggca ttttgccttc ctgtttttgc tcacccagaa acgctggtga aagtaaaaga
3781 tgctgaagat cagttgggtg cacgagtggg ttacatcgaa ctggatctca acagcggtaa
3841 gatccttgag agttttcgcc ccgaagaacg ttttccaatg atgagcactt ttaaagttct
3901 gctatgtggc gcggtattat cccgtattga cgccgggcaa gagcaactcg gtcgccgcat
3961 acactattct cagaatgact tggttgagta ctcaccagtc acagaaaagc atcttacgga
4021 tggcatgaca gtaagagaat tatgcagtgc tgccataacc atgagtgata acactgcggc
4081 caacttactt ctgacaacga tcggaggacc gaaggagcta accgcttttt tgcacaacat
4141 gggggatcat gtaactcgcc ttgatcgttg ggaaccggag ctgaatgaag ccataccaaa
4201 cgacgagcgt gacaccacga tgcctgtagc aatggcaaca acgttgcgca aactattaac
4261 tggcgaacta cttactctag cttcccggca acaattaata gactggatgg aggcggataa
4321 agttgcagga ccacttctgc gctcggccct tccggctggc tggtttattg ctgataaatc
4381 tggagccggt gagcgtgggt ctcgcggtat cattgcagca ctggggccag atggtaagcc
4441 ctcccgtatc gtagttatct acacgacggg gagtcaggca actatggatg aacgaaatag
4501 acagatcgct gagataggtg cctcactgat taagcattgg taactgtcag accaagttta
4561 ctcatatata ctttagattg atttaaaact tcatttttaa tttaaaagga tctaggtgaa
4621 gatccttttt gataatctca tgaccaaaat cccttaacgt gagttttcgt tccactgagc
4681 gtcagacccc gtagaaaaga tcaaaggatc ttcttgagat cctttttttc tgcgcgtaat
4741 ctgctgcttg caaacaaaaa aaccaccgct accagcggtg gtttgtttgc cggatcaaga
4801 gctaccaact ctttttccga aggtaactgg cttcagcaga gcgcagatac caaatactgt
4861 ccttctagtg tagccgtagt taggccacca cttcaagaac tctgtagcac cgcctacata
4921 cctcgctctg ctaatcctgt taccagtggc tgctgccagt ggcgataagt cgtgtcttac
4981 cgggttggac tcaagacgat agttaccgga taaggcgcag cggtcgggct gaacgggggg
5041 ttcgtgcaca cagcccagct tggagcgaac gacctacacc gaactgagat acctacagcg
5101 tgagctatga gaaagcgcca cgcttcccga agggagaaag gcggacaggt atccggtaag
5161 cggcagggtc ggaacaggag agcgcacgag ggagcttcca gggggaaacg cctggtatct
5221 ttatagtcct gtcgggtttc gccacctctg acttgagcgt cgatttttgt gatgctcgtc
5281 aggggggcgg agcctatgga aaaacgccag caacgcggcc tttttacggt tcctggcctt
5341 ttgctggcct tttgctcaca tgttctttcc tgcgttatcc cctgattctg tggataaccg
5401 tattaccgcc tttgagtgag ctgataccgc tcgccgcagc cgaacgaccg agcgcagcga
5461 gtcagtgagc gaggaagcgg aagagcgccc aatacgcaaa ccgcctctcc ccgcgcgttg
5521 gccgattcat taatgcag
//
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pBacPAK8载体
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