qq-plot Search Results


90
GraphPad Software Inc qq plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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GraphPad Software Inc data distribution analysis qq plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Data Distribution Analysis Qq Plot, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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BioCarta qq-plot of wks using
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot Of Wks Using, supplied by BioCarta, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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GraphPad Software Inc normal qq plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Normal Qq Plot, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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GraphPad Software Inc qq plot analysis graphpad prism 6.03
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot Analysis Graphpad Prism 6.03, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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BioCarta qq-plot of pharaoh using
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot Of Pharaoh Using, supplied by BioCarta, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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GraphPad Software Inc histogram and qq plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Histogram And Qq Plot, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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GraphPad Software Inc lognormality qq plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Lognormality Qq Plot, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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BioCarta qq-plot of drb using
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot Of Drb Using, supplied by BioCarta, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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ProMIS Neurosciences qq-plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot, supplied by ProMIS Neurosciences, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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GraphPad Software Inc lognormality qq plot and shapiro–wilk test
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Lognormality Qq Plot And Shapiro–Wilk Test, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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86
Wolters Kluwer Health qq plot
Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal <t>QQ</t> <t>plot</t> of the relative amount of the RC DNAs.
Qq Plot, supplied by Wolters Kluwer Health, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal QQ plot of the relative amount of the RC DNAs.

Journal: Frontiers in Microbiology

Article Title: DNA Engineering and Hepatitis B Virus Replication

doi: 10.3389/fmicb.2021.783040

Figure Lengend Snippet: Identification of two regions suitable for engineering. (A) Sequences that were deleted in different constructs. Deletion variants were named according to the sequences deleted. The black cycle and black triangle represent the start codon and the stop codon, respectively. The hybridization probe is shown (1199–1814). (B) The mutations of pCH9-Δε. Sequence from 1858 to 1863 was deleted, and two additional mutations, G1877T and T1878A, were introduced. (C) Representative Southern blotting of the deletion variants. The plus sign (+) denotes Eco RI digestion. RC, DL, SS DNA, and Eco RI digested fragments are indicated, respectively. (D) The relative intensity of RC DNA of deletion variants. The intensity of RC DNA of each sample was divided into the sum of RC DNA of all samples in the same membrane, respectively, to calculate the relative amount of RC DNA. N = 5. Asterisks (*) denote the difference between a deletion variant and pCH9-G2016T is statistically significant ( p < 0.05). (E) Normal QQ plot of the relative amount of the RC DNAs.

Article Snippet: QQ PLOT was used to determine the frequency distribution of the data analyzed using GraphPad Prism 8 (GraphPad Software, United States).

Techniques: Construct, Hybridization, Sequencing, Southern Blot, Membrane, Variant Assay

RNA assay of the deletion variants. (A) The sequence of HBV transcripts. The wave lines represent RNA; the black rectangles represent 5′ cap; the multiple arrowheads represent the poly-A tail. The black cycles and black triangles represent the start codon and the stop codon, respectively. The length of each transcript is an estimation without a poly-A tail. (B) Representative Northern blotting results of the deletion variants. (C) The relative intensity of pgRNA of the deletion variants. The intensity of each pgRNA/18s rRNA was divided into the sum of pgRNA/18s rRNA of all samples in the same membrane, respectively, to calculate the relative intensity of pgRNA of each sample. N = 4. Asterisks (*) denote the difference between deletion variants and pCH9-G2016T is significant ( p < 0.05). (D) Normal QQ plot of the relative amount of the pgRNAs.

Journal: Frontiers in Microbiology

Article Title: DNA Engineering and Hepatitis B Virus Replication

doi: 10.3389/fmicb.2021.783040

Figure Lengend Snippet: RNA assay of the deletion variants. (A) The sequence of HBV transcripts. The wave lines represent RNA; the black rectangles represent 5′ cap; the multiple arrowheads represent the poly-A tail. The black cycles and black triangles represent the start codon and the stop codon, respectively. The length of each transcript is an estimation without a poly-A tail. (B) Representative Northern blotting results of the deletion variants. (C) The relative intensity of pgRNA of the deletion variants. The intensity of each pgRNA/18s rRNA was divided into the sum of pgRNA/18s rRNA of all samples in the same membrane, respectively, to calculate the relative intensity of pgRNA of each sample. N = 4. Asterisks (*) denote the difference between deletion variants and pCH9-G2016T is significant ( p < 0.05). (D) Normal QQ plot of the relative amount of the pgRNAs.

Article Snippet: QQ PLOT was used to determine the frequency distribution of the data analyzed using GraphPad Prism 8 (GraphPad Software, United States).

Techniques: Sequencing, Northern Blot, Membrane